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SYSTEMS, METHODS AND COMPOSITION OF USING RNASE III MUTANTS TO PRODUCE SRNA TO CONTROL HOST PATHOGEN INFECTION

20230354822 · 2023-11-09

    Inventors

    Cpc classification

    International classification

    Abstract

    The current invention includes systems, methods and compositions for the generation of sRNA molecules using select RNase III mutants. In one preferred embodiment, invention includes systems, methods and compositions for the generation of sRNA molecules using RNase III mutants to control a host pathogen through the production and diffusion of sRNA molecules that may initiate an RNAi pathway response directed to a host pathogen. Additional embodiments of the current invention include systems, methods and compositions for the DICER-independent generation of sRNA molecules using select RNase III mutants.

    Claims

    1. Genetically modified bacteria engineered to co-express a heterologous bacterial RNase III mutant and a heterologous target dsRNA molecule, wherein said target dsRNA molecule is directed to an essential gene of a target pathogen, pest, or herbivore, wherein said RNase III mutant upon expression cleaves said target dsRNA molecule into sRNA molecules of a discrete size capable of inducing RNA silencing in said target pathogen, pest, or herbivore.

    2. The genetically modified bacteria of claim 1, wherein said genetically modified bacteria is configured for introduction to a target host that is susceptible to said pathogen, pest, or herbivore.

    3. The genetically modified bacteria of claim 2, wherein said genetically modified bacteria is a symbiotic and/or endosymbiotic bacteria with said target host.

    4. The genetically modified bacteria of claim 2, wherein said target host is a plant host or an animal host.

    5. The genetically modified bacteria of claim 2, wherein said sRNA molecules of a discrete size are generated by said genetically modified bacteria and delivered to said target host or directly to said target pathogen, pest, or herbivore to induce an RNAi pathway response in said target pathogen, pest, or herbivore and protect the target host from said target pathogen, pest, or herbivore.

    6. The genetically modified bacteria of claim 1, wherein said genetically modified bacteria comprises a heterologous polynucleotide encoding said heterologous bacterial RNase III mutant and a heterologous polynucleotide encoding said heterologous target dsRNA molecule.

    7. The genetically modified bacteria of claim 1, wherein said sRNA molecules of a discrete size consist of 22 to 23 nucleotides (nt).

    8. The genetically modified bacteria of claim 1, heterologous bacterial RNase III mutant is derived from a wild type RNase III from a bacteria selected from the group consisting of: E. coli, Enterobacter sp., Bacillus sp., S. enterica, P. aeruginosa, C. burnetii, R. capsulatus, S. coelicolor, C. jejuni, H. pylori, S. aureus, and L. lactis.

    9. The genetically modified bacteria of claim 1, wherein said essential gene is an essential viral pathogen gene.

    10. A composition for initiating RNA interference (RNAi) in a target pathogen, pest, or herbivore, said composition comprising a plurality of genetically modified bacteria according to claim 1 dispersed in a carrier.

    11. The composition of claim 10, wherein said composition is a wettable powder, spray, emulsion, colloid, aqueous or organic solution, dust, pellet, or colloidal concentrate.

    12. The composition of claim 10, wherein said composition is a liquid solution, foam, suspension, or emulsifiable concentrate.

    13. The composition of claim 10, wherein composition is an animal feed.

    14. The composition of claim 10, further comprising powdered corncobs, rice hulls, and/or walnut shells.

    15. A method of initiating RNA interference (RNAi) in a target pathogen, pest, or herbivore, the method comprising: administering or applying to a target host an effective amount of a genetically modified bacteria according to claim 1, wherein said target host is infected with or susceptible to said target pathogen, pest, or herbivore; wherein said genetically modified bacteria expresses said RNase III mutant that cleaves said co-expressed target dsRNA molecule into sRNA molecules of a discrete size, wherein said sRNA molecules of discrete size are generated by said genetically modified bacteria and delivered to said target host or directly to said target pathogen, pest, or herbivore to induce an RNAi pathway response in said target pathogen, pest, or herbivore and protect said target host from said target pathogen, pest, or herbivore.

    16. The method of claim 15, wherein said sRNA molecules downregulate said essential gene of said target pathogen, pest, or herbivore pathogen through said a DICER-independent RNAi response pathway.

    17. The method of claim 15, wherein said administering or applying comprises feeding said effective amount of said genetically modified bacteria to said target host.

    18. The method of claim 15, wherein said administering or applying comprises applying said effective amount of said genetically modified bacteria to a target host plant topically.

    19. The method of claim 15, wherein said genetically modified bacteria is administered or applied prophylactically.

    20. The method of claim 15, wherein said sRNA molecules of discrete size consist of 22 to 23 nucleotides.

    Description

    BRIEF DESCRIPTION OF THE FIGURES

    [0254] The above and other aspects, features, and advantages of the present disclosure will be better understood from the following detailed descriptions taken in conjunction with the accompanying figures, all of which are given by way of illustration only, and are not limiting the presently disclosed embodiments, in which:

    [0255] FIG. 1A: The catalytic centers of E. coli Ribonuclease III (RNase III).

    [0256] FIG. 1B: Homologous recombination to directly make bacterial RNase III point mutant (tet-sacB counter selection) in the bacterial chromosome.

    [0257] FIG. 2: The identification of pKD46 and pSIJ8 plasmids by digestion with EcoRI-HF® restriction enzyme. Lane M: 1 kb DNA ladder; lanes 1-2: pKD46 digested with EcoRI-HF® restriction enzyme, and the expected fragment sizes are ˜4.8 kb and ˜1.5 kb; lanes 3-4: pSIJ8 digested with EcoRT-HF® restriction enzyme, and the expected fragment sizes are ˜0.8 kb, 1.3 kb, ˜1.5 kb, and ˜6.0 kb.

    [0258] FIG. 3: PCR amplification of tetA-sacB cassette inserted into E. coli JM109 (DE3) RNase III E38 and E117K positions. Lane M: 100 bp DNA ladder; lanes 1-7: PCR amplification of tetA-sacB cassette inserted into E. coli JM109 (DE3) RNase III E38 position with primers JD-5 and Tet-sacB-JD-R1, and the expected fragment size is 368 bp; lanes 8-14: PCR amplification of tetA-sacB cassette inserted into E. coli JM109 (DE3) RNase III E117 position with primers JD-5 and Tet-sacB-JD-R1, and the expected fragment size is 605 bp.

    [0259] FIG. 4: Screening of E38A-L40F and E117K-L119F mutants. Lane M: 100 bp DNA ladder; lanes 1-7: PCR amplification of E. coli JM109 (DE3) RNase III E38A-L40F candidate mutants with primers Ecoli-E38A-1F and Ecoli-E38A-1R, and the expected fragment size is 256 bp; lanes 8-14: PCR amplification of E. coli JM109 (DE3) RNase III E117K-L119F candidate mutants with primers Ecoli-E117K-1F and Ecoli-E117K-1R, and the expected fragment size is 323 bp; lanes 15-21: PCR amplification of the same E. coli JM109 (DE3) RNase III E38A-L40F candidate mutants in lanes 1-7 with primers JD-5 and JD-3, and the expected fragment size is 879 bp; lanes 22-28: PCR amplification of the same E. coli JM109 (DE3) RNase III E117K-L119F candidate mutants in lanes 8-14 with primers JD-5 and JD-3, and the expected fragment size is 879 bp.

    [0260] FIG. 5: Screening of E38A and E117K mutants. Lane M: 100 bp DNA ladder; lanes1, 3, and 5: PCR amplification E. coli JM109 (DE3) RNase III E38A mutants with primers Ecoli-E38A-2F and Ecoli-E38A-1R, and the expected fragment size is 256 bp; lanes 2, 4, and 6: PCR amplification of the same possible E. coli JM109 (DE3) RNase III E38A-L40F mutants in lanes 1, 3, and 5 with primers JD-5 and JD-3, and the expected fragment size is 879 bp; lanes 7, 9, and 11: PCR amplification E. coli JM109 (DE3) RNase III E117K mutants with primers Ecoli-E117K-2F and Ecoli-E117K-1R, and the expected fragment size is 323 bp; lanes 8, 10, and 12: PCR amplification of the same possible E. coli JM109 (DE3) RNase III E117K mutants in lanes 7, 9, and 11 with primers JD-5 and JD-3, and the expected fragment size is 879 bp.

    [0261] FIG. 6: Screening of E65A mutant. Lane M: 100 bp DNA ladder; lanes1-3, PCR amplification of E. coli JM109 (DE3) RNase III E65<tetA-sacB> mutant with primers JD-5 and Tet-sacB-JD-R1, and the expected fragment size is 449 bp; lanes 4, 6, 8, 10, 12, 14, and 16: PCR amplification of E. coli JM109 (DE3) RNase III candidate E65A mutants with primers Ecoli-E65A-1F and JD-3, and the expected fragment size is 604 bp; lanes 5, 7, 9, 11, 13, 15, and 17: PCR amplification of the same E. coli JM109 (DE3) candidate RNase III 65A mutants in lanes 4, 6, 8, 10, 12, 14, and 16 with primers JD-5 and JD-3, and the expected fragment size is 879 bp.

    [0262] FIG. 7: Bc-E58A and Bc-E137K mutant construction. Lane M: 100 bp DNA ladder; lanes 1-2: PCR amplification using Pveg plasmid as template with primers Pveg-F1 and Pveg-R1, and the expected PCR size is 273 bp; lanes 3-6: PCR amplification using the genomic DNA of B. cereus 53522 as template with primers Bc-E58A-F1 and Bc-E58A-R1, and the expected PCR fragment size is 205 bp; lanes 7-10: PCR amplification using the genomic DNA of B. cereus 53522 as template with primers Bc-E58A-F2 and Bc-E58A-R2, and the expected PCR fragment size is 608 bp; lanes 11-14: PCR amplification using the genomic DNA of B. cereus 53522 as template with primers Bc-E58A-F1 and Bc-E137K-R1, and the expected PCR fragment size is 445 bp; lanes 15-18: PCR amplification using the genomic DNA of B. cereus 53522 as template with primers Bc-E137K-F1 and Bc-E58A-R2, and the expected PCR fragment size is 368 bp.

    [0263] FIG. 8: Construction of the pAD-WRKY-GHY7-Pveg3 plasmid. Lane M: GeneRuler DNA Ladder Mix; lane 1: pAD-WRKY-GHY7 was digested with EcoRI-HF® restriction enzyme, and the expected fragment size is ˜7.2 kb; lane 2: PCR amplification with primers Pveg-F2 and Pveg-R2 using Pveg plasmid as template, and the expected fragment size is 273 bp; lanes 3-4: pAD-WRKY-GHY7-Pveg3 plasmid was digested with XhoI and the expected fragment size is ˜7.5 kb.

    [0264] FIG. 9: PCR screening of the predicted RNase III mutants. Lane M: 100 bp DNA ladder; lanes 1-7: PCR amplification of HT115-Bs(Bacillus subtilis)-E59A mutants; lanes 8-10: PCR amplification of HT115-Bs-E138K mutants; lanes 11-13: PCR amplification of HT115-Ec-E38A-ΔSA mutants; lanes 14-16: PCR amplification of HT115-Ec-E38A-ΔSASS mutants; lanes 17-19: PCR amplification of HT115-Ec-E38A-ΔSA-ΔGPG mutants; lanes 20-21: PCR amplification of HT115-Ec-E38A-ΔSASS-ΔGPG mutants; lanes 23-25: PCR amplification of HT115-Ec-E38A-R107A-R108A mutants; lanes 26-28: PCR amplification of HT115-Ec-E38A-R107E-R108E mutants; lanes 29-30: PCR amplification of HT115-Ec-ΔSASS-ΔGPG mutants.

    [0265] FIG. 10: The mc gene of Enterobacteria Ae003, Ae073, and Ag001. Lane M: 100 bp DNA ladder; lane 1: PCR amplification of Ae003 with Ae-JD-5 and Ae-JD-3 primers, and the expected fragment size is ˜1.2 kb; lane 2: PCR amplification of Ae073 with Ae-JD-5 and Ae-JD-3 primers, and the expected fragment size is ˜1.2 kb; lane 3: PCR amplification of Ag001 with Ae-JD-5 and Ae-JD-3 primer identification, and the expected fragment size is ˜1.2 kb.

    [0266] FIG. 11: PCR screening of the predicted RNase III mutants. Lane M: 100 bp DNA ladder; lanes 1-6: PCR amplification of HT115-Ae003-E38A mutants; lanes 7-14: PCR amplification of HT115-E38A-ΔS33-ΔS34-ΔK35 mutants; lanes 15-21: PCR amplification of HT115-Ag001-E38A-R107A-R108A mutant; lanes 22-28: PCR amplification of HT115-E30A mutant; lanes 29-35: PCR amplification of HT115-E38A-ΔA32-ΔS33-ΔS34-K35V mutants; lanes 36-42: PCR amplification of HT115-E38A-K12opt mutants; lanes 43-47: PCR amplification of HT115-E117D.

    [0267] FIG. 12: PCR screening of the predicted RNase III mutants. Lane M: 100 bp DNA ladder; lanes 1-6: PCR amplification of HT115-E38A-ΔA32-ΔS33-ΔS34 mutants; lanes 7-12: PCR amplification of HT115-E38A-ΔS33-R107A-R108A mutants; lanes 13-18: PCR amplification of HT115-E38A-S33A-ΔS34-R107A-R108A mutants; lanes 19-24: PCR amplification of HT115-Ag001-E38A mutants; lanes 25-30: PCR amplification of HT115-Ae003-E38A-R107A-R108A mutants; lanes 31-36: PCR amplification of HT115-E30A-K12opt mutants; lanes 37-42: PCR amplification of HT115-E117Q mutants; lanes 43-48: PCR amplification of HT115-Q153P mutants; lanes 49-54: PCR amplification of HT115-D155E mutants.

    [0268] FIG. 13: Northern blot revealing small interfering RNA molecules of 23 nucleotides (upper panel). GelGreen® Nucleic Acid-stained rRNA served as loading controls in the gel prior to RNA transfer (lower panel). 6 μg total small RNA was loaded per well. Lane 1: The dsRNA extracted from HT115(DE3) (RNase III mutant) containing pAD-WRKY-GHY7 plasmid (TMV movement protein sRNA, and specifically a hpRNA), negative control; Lane 2: The dsRNA extracted from JM109 (wide-type E. coli) containing pAD-WRKY-GHY7 plasmid, negative control; Lane 3: The siRNA extracted from JM109 (wide-type E. coli) containing pAD-WRKY-GHY7 plasmid, negative control; Lane 4: The siRNA extracted from predicted mutant HT115-E38A-ΔSA; Lane 5: The siRNA extracted from predicted mutant HT115-E38A-ΔSASS; Lane 6: The siRNA extracted from predicted mutant HT115-E38A-ΔSA-ΔGPG; Lane 7: The siRNA extracted from predicted mutant HT115-E38A-ΔSASS-ΔGPG; Lane 8: The siRNA extracted from predicted mutant HT115-E38A-R107A-R108A; Lane 9: The siRNA extracted from predicted mutant HT115-E38A-R107E-R108E; Lane 9: The siRNA extracted from predicted mutant HT115-Ec-ΔSASS-ΔGPG.

    [0269] FIG. 14: Northern blot revealing small RNA nucleotides. 5 μg total small RNA was loaded per well. Lanes M: TMV movement protein gene specific single-stranded RNA marker and it consists of five ssRNA: 21, 23, 25, 27 and 29 bases. Lane 1: TMV movement protein gene specific single-stranded RNA marker, 21 base; Lanes 2-3: The total small RNAs extracted from wide-type E. coli JM109 (DE3); Lanes 4-5: The total small RNAs extracted from wide-type E. coli JM109 (DE3) containing pAD-WRKY-GHY7 plasmid; Lanes 6-7: The total small RNAs extracted from HT115-E38A-GHY7 (RNaseIII E38A constructed in the plasmid, code optimization with E. coli K12 strain); Lanes 8-9: The total small RNAs extracted from E. coli E65A mutant containing pAD-WRKY-GHY7 plasmid; Lanes 10-11: The total small RNAs extracted from HT115-E38A-R107A-R108A.

    [0270] FIG. 15: Northern blot revealing small interfering RNA molecules of 23 nucleotides (upper panel). GelGreen® Nucleic Acid-stained rRNA served as loading controls in the gel prior to RNA transfer (lower panel). 6 μg total small RNA was loaded per well. Lane 1: The siRNA extracted from E38A-L40F mutant containing pAD-WRKY-GHY7 plasmid (TMV movement protein hpRNA), positive control; Lanes 2-3: The siRNA extracted from predicted mutant HT115-E38A-ΔSA; Lanes 4-5: The siRNA extracted from predicted mutant HT115-E38A-ΔSASS; Lanes 6-7: The siRNA extracted from predicted mutant HT115-E38A-MA-ΔGPG; Lanes 8-9: The siRNA extracted from predicted mutant HT115-E38A-ΔSASS-ΔGPG; Lanes 10-11: The siRNA extracted from predicted mutant HT115-E38A R107E-R108E.

    [0271] FIG. 16: qRT-PCR of dsRNA cleavage from different E. coli RNase III mutants.* indicates P<0.05. HT115-pAD-WRKY-GHY7: HT115 strain containing pAD-WRKY-GHY7 plasmid (tetracycline and chloramphenicol resistance), and it cannot digest dsRNA; HT115-pAD-WRKY-GHY7-E38A: HT115 strain containing pAD-WRKY-GHY7-E38A plasmid (tetracycline and chloramphenicol resistance), and E38A RNaseIII mutant can digest dsRNA into 26-29 bp small RNA; this strain can convert almost half of dsRNA into small RNAs compared to HT115-pAD-WRKY-GHY7, which cannot digest the dsRNA molecules; JM109-pAD-WRKY-GHY7: JM109 (DE3) RNaseIII E38A mutant containing pAD-WRKY-GHY7 plasmid (chloramphenicol resistance), it can cleave dsRNA into 26-29 bp small RNA; this strain can convert almost 85% dsRNA into small RNAs compared to HT115-pAD-WRKY-GHY7. HT115-E38A-R107A-R108A: HT115 strain containing pAD-WRKY-GHY7-E38A-R107A-R108A plasmid (tetracycline and chloramphenicol resistance), and it can effectively cleave dsRNA into 22-23 bp small RNA; it can convert almost 95% dsRNA into small RNAs compared to HT115-pAD-WRKY-GHY7; HT115-E38A-R107E-R108E: HT115 strain containing pAD-WRKY-GHY7-E38A-R107E-R108E plasmid (tetracycline and chloramphenicol resistance), and it can cleave dsRNA into 26-29 bp small RNA and can convert almost 80% dsRNA into small RNA compared to HT115-pAD-WRKY-GHY7-E38A.

    [0272] FIG. 17: Northern blot revealing small interfering RNA molecules of 23 nucleotides (upper panel). GelGreen® Nucleic Acid-stained RNA indicated the RNA bands in the gel prior to RNA transfer. 12 μg total small RNA was loaded per well. 18 nM TMV movement protein gene-specific DNA primers (21 nt) mixed with dsRNA Ladder (NEB) was used to indicate 21 nt. Lanes 1-2: The total siRNAs extracted from HT115-E38A (RNase III mutant, code optimization with E. coli K12 strain), positive control; Lanes 3-4: The total siRNAs extracted from HT115-Ae003-E38A, and this is to check if Enterobacteria RNase III E38A mutant shows similar dsRNA cleavage like E. coli strains; Lanes 5-6: The total siRNAs extracted from HT115-Ag001-E38A-R107A-R108A, and this is to check if this mutant shows similar dsRNA cleavage like E. coli E38A-R107A-R108A mutant; Lane 7: The total siRNAs extracted from HT115-Ag001-E38A-R86C-R107A-R108A, and this is to check if this mutant shows similar dsRNA cleavage like E. coli E38A-R107A-R108A mutant; Lane 8: The total siRNAs extracted from HT115-ver-E30A, the Verrucomicrobia bacterium E30A RNase III mutant, dsRNA cleavage is supposed to be similar to E. coli E38A mutant; Lanes 9-10: The total siRNA extracted from predicted mutant HT115-E38A-ΔS33-ΔS34-ΔK35; Lanes 11-12: The total siRNA extracted from predicted mutant HT115-E38A-ΔA32-ΔS33-ΔS34-K35; Lane 13: The total siRNA extracted from wide-type bacterial strain JM109 (DE3), negative control; Lane 14: The total siRNA extracted from RNase III mutant HT115 (DE3), negative control.

    [0273] FIG. 18: Northern blot revealing small interfering RNA molecules of 22-23 nucleotides. 12 μg total small RNA was loaded per well. 6 nM TMV movement protein gene-specific DNA primers (21nt) mixed with dsRNA Ladder (NEB) was used to indicate 21 nt. Lanes 1-2: The total siRNAs extracted from predicted mutant HT115-Ec-E38A-ΔA32-ΔS33-ΔS34; Lanes 3-4: The total siRNAs extracted from predicted mutant HT115-Ec-E38A-ΔS33-R107A-R108A; Lanes 5-6: The total siRNAs extracted from predicted mutant HT115-Ec-E38A-S33A-ΔS34-R107A-R108A; Lanes 7-8: The total siRNA extracted from Ag001-E38A and this mutant produced 26-29 nt siRNA; this is to check if this mutant shows similar dsRNA cleavage like E. coli Ec-E38A mutant; Lanes 9-10: The total siRNAs extracted from HT115-Ae003-E38A-R107A-R108A, and this mutant produced 22-23 nt siRNA; this is to check if this mutant shows similar dsRNA cleavage like E. coli-E38A-R107A-R108A mutant; Lanes 11-12: The total siRNAs extracted from HT115-ver-E30A-K12opt, the Verrucomicrobia bacterium E3 OA RNase III mutant with code optimization.

    [0274] FIG. 19: Homology model of WT E. coli RNase III dimer (green and blue cartoons) based on a crystal structure of WT A. aeolicus RNase III (light green and cyan cartoons). Bound dsRNA is shown in the center as orange cartoons. Note the high structural overlap of the E. coli model with the A. aeolicus structure, particularly at secondary structural elements (a-helices and β-sheets). For clarity, bound magnesium ions are not shown.

    [0275] FIG. 20: Close-up of binding interface in the homology model of WT E. coli RNase III dimer (green and blue cartoons). Bound dsRNA is shown as orange cartoons. E38 from one monomer and E65 from the other monomer are shown as sticks. The carboxyl groups of both anionic side chains are pointing towards the negatively-charged backbone of the bound dsRNA, which can lead to electrostatic repulsions at the binding interface. Yellow dashed lines give the distance (in Angstroms) between each side chain and the dsRNA backbone. Note that the E65 side chain is positioned closer to the dsRNA backbone. For clarity, bound magnesium ions are not shown.

    [0276] FIG. 21A-B: Correlation between predicted dsRNA-binding free energy of E. coli RNase III and its cutting efficiency (based on experimental measurements of the proportion of aligned sRNA reads). The left plot (A) shows the correlation using non-relative values on both axes (y-axis here gives ΔG binding), while the right plot (B) gives the corresponding correlation when both axes are taken relative to WT values (y-axis here gives ΔΔG binding relative to WT). Blue squares represent data points for individual experimental measurements (see Table 1); the point mutations for these data points are given to the right in black text. A trend line was calculated for these data points in both plots, with the R.sup.2 of the linear fit given at the lower-left of each plot. Note the high linear correlation observed in both plots. Orange diamonds represent predictions for particular RNase III mutants that are still being tested; the point mutations for these constructs are given to the right in red text.

    [0277] FIG. 22: Structural model of two E. coli WT RNase III dimers (green and blue cartoons) separated by 26 nt along a dsRNA target. Note that at this separation, both dimers are not showing steric clashes with each other, as indicated by the absence of any overlaps between their van der Waals (i.e., molecular) surfaces. Yellow and red RNA strands represent the 26-nt long dsRNA cleavage product, while white RNA strands denote the rest of the dsRNA target. For clarity, bound magnesium ions are not shown.

    [0278] FIG. 23: Structural model of two E. coli E38A/R107A/R108A mutant RNase III dimers (green and blue cartoons) separated by 22 nt along a dsRNA target. Note that at this separation, both dimers are not showing steric clashes with each other, as indicated by the absence of any overlaps between their van der Waals (i.e., molecular) surfaces. Yellow and red RNA strands represent the 22-nt long dsRNA cleavage product, while white RNA strands denote the rest of the dsRNA target. For clarity, bound magnesium ions are not shown.

    [0279] FIG. 24A-R: Size distributions of sRNA 18nt-30nt (Fixed Y) for multiple RNase III mutants: FIG. 24A-B, A. E38A-GHY7-1 and B. E38A-GHY7-2; FIG. 24C-D, C. E38A-GHY7-3 and D. E65A-GHY7-1; FIG. 24E-F, E. E65A-GHY7-2 and F. E65A-GHY7-3; FIG. 24G-H, G. E38A-R107A-R108A-GHY7-1 and H. E38A-R107A-R108A-GHY7-2; FIG. 24I, I. E38A-R107A-R108A-GHY7-3; FIG. 24J-K, J. E38A-R107E-R108E-GHY7-1 and K. E38A-R107E-R108E-GHY7-2; FIG. 24L-M, L. E38A-R107E-R108E-GHY7-3 and M. JM109-GHY7-1; FIG. 24N-O, N. JM109-GHY7-2 and O. JM109-GHY7-3; FIG. 24P-Q, P. JM109-1 and Q. JM109-2; and FIG. 24R, R. JM109-2.

    [0280] FIG. 25A-O: Coverage mapping to GHY7 construct of sRNA 18nt-30nt.

    [0281] FIG. 26: Unconstrained ordination of sRNA populations in each sample.

    [0282] FIG. 27: Shannon Diversity index scores of sRNA populations.

    [0283] FIG. 28: Northern blot revealing small RNA nucleotides. 6 μg total small RNA was loaded per well. Lanes M: TMV movement protein gene specific single-stranded RNA marker and it consists of five ssRNA: 21, 23, 25, 27 and 29 bases. Lane 1: TMV movement protein gene specific single-stranded RNA marker, 21 base; Lane 2: The total small RNAs extracted from HT115-E38A-R107A-R108A, and 5 ug loaded; Lane 3: The total small RNAs extracted from HT115-Bc-E58A; Lane 4: The total small RNAs extracted from HT115-Bs-E59A; Lane 5: The total small RNAs extracted from HT115-Ec-E117D; Lane 6: The total small RNAs extracted from HT115-Ec-E117Q; Lane 7: The total small RNAs extracted from HT115-Ec-Q153P; Lane 8: The total small RNAs extracted from HT115-Ec-D155E; Lane 9: The total small RNAs extracted from HT115-Bc-E138K; Lane 10: The total small RNAs extracted from E. coli mutant E117K containing pAD-WRKY-GHY7 plasmid; Lane 10: The total small RNAs extracted from E. coli mutant E117K-L119F containing pAD-WRKY-GHY7 plasmid.

    MODE(S) FOR CARRYING OUT THE INVENTION(S)

    [0284] The following detailed description is provided to aid those skilled in the art in practicing the various embodiments of the present disclosure, including all the methods, uses, compositions, etc., described herein. Even so, the following detailed description should not be construed to unduly limit the present disclosure, as modifications and variations in the embodiments herein discussed may be made by those of ordinary skill in the art without departing from the spirit or scope of the present discoveries. The present disclosure is explained in greater detail below. This disclosure is not intended to be a detailed catalog of all the different ways in which embodiments of this disclosure can be implemented, or all the features that can be added to the instant embodiments. For example, features illustrated with respect to one embodiment may be incorporated into other embodiments, and features illustrated with respect to a particular embodiment may be deleted from that embodiment. In addition, numerous variations and additions to the various embodiments suggested herein will be apparent to those skilled in the art in light of the instant disclosure, which variations and additions do not depart from the scope of the instant disclosure. Hence, the following specification is intended to illustrate some particular embodiments of the disclosure, and not to exhaustively specify all permutations, combinations, and variations thereof.

    [0285] As shown in the figures, in one embodiment, mutations in an RNase III protein identified herein may result in the stabilization of RNase III cutting patterns leading to more consistent dsRNA cutting. As used herein, the term consistent dsRNA cutting, generally refer to the RNase III mutant protein's ability to produce relatively more sRNA products of a specific size and less relative undesirable sRNA of off-target sizes. This may be demonstrated by effectively narrowing the distribution of sRNA in the population around a specific peak as generally demonstrated in FIG. 24A-R and Table 7. The present inventors have demonstrated that this “consistent dsRNA cutting” effect also results in a more consistent cutting profile of sRNA by not stochastically shifting the cutting “ladder” of the protein with each cut as would be expected to occur in a wider sRNA size distribution such as that from the wild-type RNase III or DICER. The ultimate result of these factors is more predictable cutting and sequence-based end products in a final heterologous sRNA population measurable as a decrease in population diversity.

    [0286] In another embodiment, the present inventors demonstrate that the current literature potentially misinterprets E38A as a mutant RNase III that cuts a preferred 23 nt pattern. Xiao et al. originally characterized dsRNA cutting by the E38A mutant to prefer producing 23n t sRNA (Xiao et al. 2009). This finding was based on northern analysis techniques lack enough resolution to call fragment sizes accurately to the specific base pair (Doran et al. 1999). Modern sequencing technologies can vastly improve size evaluation by looking at the actual sequence of sRNA reads to get an accurate length.

    [0287] The present inventors performed high throughput sRNA sequencing using the Illumina Hi-Seq platform as outlined in sRNA Analysis methods. As shown in FIG. 24A-R, the present inventors identified that E38A's preferred cutting length is actually 26 nt. The size distribution of E38A is actually highly similar to that of the wild-type with a peak at 26 nt. However, wildtype has another peak at 29 nt not see as prevalently in E38A.

    [0288] As further demonstrated in FIG. 25A-O, the preferred cutting locations along the exemplary sRNA from Tobacco mosaic virus (TMV) GHY7 dsRNA sequence are also very similar to those of the wildtype (JM109). Populations of sRNA in E38A and wildtype did not differ significantly in pairwise analysis (via DMRT). However, E38A did differ significantly in terms of relative abundance of sRNA in the 18-30 nt range when compared to wildtype (DMRT, stat=2.19, p=0.014). These findings demonstrate that E38A, rather than primarily making discrete cuts at 23 nt, instead acts as a catalytic efficiency mutant producing approximately 3× more sRNA than wildtype as shown in Table 5. As also demonstrated in FIG. 20, the mutation E38A is changing a strongly negative residue to a hydrophobic one which may increases the binding affinity with dsRNA. As further shown in FIG. 21A-B, estimation of binding free energies using the MM-GBSA computational technique indeed shows that mutation E38A causes the RNase III dimer to bind more stably to dsRNA (compared to WT).

    [0289] As generally shown in FIG. 22, structural modeling of two E. coli WT RNase III dimers on a dsRNA target indicate that with a separation of 26 nt, both RNase III are separated far enough to not cause steric clashes and thus to not interfere with each other. Structural models also show no steric clashes between both RNase III dimers when separated by 23 nt.

    [0290] The present inventors further demonstrate that a new RNase III mutant, E65A, is more catalytically efficient than both E38A and wildtype RNase III. Generally referring to FIG. 20, the E38 and E65 residues of RNase III are adjacent in a dimer formation of RNase III protein monomers bound to dsRNA. The empirical data show that the E65A is significantly more efficient at producing sRNA than JM109 wildtype (DMRT, stat=3.3, p<0.01) and E38A (KW, stat=3.9, p=0.049). As shown in Table 5 below, the RNase III E65A mutant is approximately 4.4× more catalytically efficient than the wildtype and approximately 1.5× more efficient than E38A. The increase in catalytic efficiency may be due to a similar mechanism as dsRNA binding affinity enhancement seen in RNase III mutant E38A. As shown in FIG. 20, the E65 side chain is positioned closer to the dsRNA backbone (compared to the E38-dsRNA distance), and so the mutation E65A may decrease the electrostatic repulsion forces at the binding interface more than the E38A mutation. As shown in FIG. 21A-B, estimation of binding free energies using the MM-GBSA computational technique indeed shows that mutation E65A causes the RNase III dimer to bind more stably to dsRNA compared to both E38A and WT.

    [0291] In another embodiment, the present inventors demonstrate that a novel RNase III mutant E38A-R107A-R108A possesses increased catalytic efficiency and differential discrete cutting when compared to wildtype (JM109). The present inventors performed sRNA analysis using methods outlined herein. The RNase III mutant E38A-R107A-R108A produced significantly different relative abundances of sRNA product than wildtype (KW, stat 3.86, p=0.049). As shown in Table 5, the increase was approximately 2.7× over wildtype (JM109). As further shown in Table 6, sRNA populations were significantly different between tested mutants and wildtypes in both PERMANOVA and ANOSIM tests. As shown in FIG. 26, NMDS analysis shows how divergent the sRNA populations are in the RNase III mutant E38A-R107A-R108A from other tested mutants and wildtype. One of the primary causes for this is the redistribution of sRNA products into what is almost exclusively 22 and 23 nt sRNA as demonstrated in FIG. 24A-R. Additionally, this represents a decrease in diversity of sRNA products, (see FIG. 27), or, a more homogenous mix of sized sRNA products of 22 and 23 nt. The RNase III mutant E38A-R107A-R108A ultimately results in fewer differentially sized products in higher quantity, desirable traits for RNAi technologies. Diversity of sRNA populations in the RNase III mutant E38A-R107A-R108A was significantly different from both E38A (DMRT, stat=2.04, p<0.0208) and the JM109 wildtype (DMRT, stat=3.06, p<0.01).

    [0292] As further demonstrated in FIG. 21A-B, estimation of binding free energies using the MM-GBSA computational technique demonstrates that triple mutation E38A/R107A/R108A causes the RNase III dimer to bind more stably to dsRNA (compared to WT). As further demonstrated in FIG. 23, structural modeling of two E. coli E38A/R107A/R108A mutant RNase III dimers on a dsRNA target indicate that with a separation of 22 nt, both RNase III are separated far enough to not cause steric clashes and thus to not interfere with each other. This observation is further generally applicable for the slightly farther separation of 23 nt.

    [0293] Further evidence of cutting changes in the RNase III mutant E38A-R107A-R108A can be shown in the cutting pattern or ladder along the GHY7 construct. As shown in FIG. 25A-O, peak regions or hot spots along the dsRNA construct, while similar in E38A, E65A, and JM109, are very different in E38A-R107A-R108A.

    [0294] Another RNase III mutant, E28A-R107E-R108E was tested in the same manner as RNase III mutant E38A-R107A-R108A. It was able to cleave dsRNA per northern analyses. However, in RNA-seq analysis, it did not demonstrate significant efficiency or cutting pattern/size differentiation from the wildtype. In this RNase III E28A-R107E-R108E mutant, the two arginine to glutamic acid mutations are replacing electrostatic attractive forces with electrostatic repulsive forces to make dsRNA binding less stable. Indeed, as shown in FIG. 21A-B, estimation of binding free energies using the MM-GBSA computational technique shows that triple mutation E38A/R107E/R108E causes reduced stability of binding by RNase III dimer to dsRNA relative to both E38A and E38A/R107A/R108A RNase III.

    [0295] In another embodiment, the present inventors demonstrate that RNase III mutant E38A-E65A is combinatorial regarding the catalytic effects of E38A and E65A. As demonstrated in FIG. 21A-B, estimation of binding free energies using the MM-GBSA computational technique predicts that mutation E38A/E65A causes the RNase III dimer to bind more stably to dsRNA (compared to E38A alone or E65A alone), although the contributions of the single mutations to increasing the binding free energy are not additive (i.e., predicted binding free energy for E38A/E65A is less than the sum of those for E38A alone and E65A alone). As a result, the E38A/E65A mutant may have high catalytic efficiency, with a preferred dsRNA cutting length of 26 nt.

    [0296] The present inventors next tested if the quadruple RNase III mutant E38A-E65A-R107A-R108A combines the predicted enhanced catalytic efficiency of E38A-E65A with the observed preferred cutting length of 22-23 nt when R107A-R108A mutations were added to E38A. Surprisingly, estimation of binding free energies using the MM-GBSA computational technique predicts that quadruple RNase III mutant E38A-E65A-R107A-R108A causes the RNase III dimer to bind less stably to dsRNA (compared to E38A or triple RNase III mutant E38A-R107A-E108A) as shown in FIG. 21A-B. Thus, the quadruple mutant may also exhibit a preferred cutting length of 22-23 nt; it may be less efficient than RNase III mutant E38A-R107A-R108A as described above at performing this cleavage of dsRNA.

    [0297] An additional test using independent MD simulations and analysis of RNase III mutant E65A-R107A-R108A shows that this tripe mutant is predicted to be comparable to WT in terms of predicted binding free energy to dsRNA (and less than those of E38A, E38A-R107A-R108A, and even E38A-R107E-R108E) (See FIG. 21A-B). It should also be noted that the predicted change in binding free energy between E38A-E65A and E38A-E65A-R107A-R108A is comparable to the change between RNase III mutants E65A and E65A-R107A-R108A (See e.g., FIG. 21A-B). As such, the present inventors demonstrate that unlike with E38A, there is more structural dialogue of R107A-R108A with E65A such that combination of these causes reduced binding free energy and thus reduced catalytic efficiency.

    [0298] As noted above, RNAi silencing mechanisms are generally reliant on sRNAs sized 21-23nt (Martinez and Richard 2013, Zamore et al. 2000). As shown generally in FIG. 24A-R and Table 7, 21 nt sRNA production was relatively the same in RNase III mutants E38A and E38A-R107A-R108A, with both producing ˜1.5× the amount the wildtype produces. However, RNase III mutant E38A-R107A-R108A produced ˜6.5× more 22 nt sRNA than E38A alone and ˜14× more than the wildtype. The present inventor further demonstrated that RNase III mutant E38A-R107A-R108A also produced ˜10.5× more 23 nt sRNA than E38A and ˜22.5× more 23 nt sRNA than wildtype.

    [0299] Each of the aforementioned RNaseIII mutants may be generally be referred to as an “RNase III mutant,” “mutant,” or by its specific amino acid mutation designation i.e. residue and location.

    [0300] One embodiment of the current invention includes systems, methods and compositions for the generation of sRNA molecules using RNase III mutants. In one preferred embodiment, invention includes systems, methods and compositions for the generation of sRNA molecules using RNase III mutants to control a host pathogen through the production and diffusion of sRNA molecules that may initiate an RNAi pathway response directed to a host pathogen. Another embodiment of the current invention includes systems, methods and compositions for the generation of sRNA molecules using RNase III mutants may be accomplished in vivo, in vitro, or ex vivo.

    [0301] Another embodiment of the current invention includes systems, methods and compositions for the generation of sRNA molecules using RNase III mutants to produce a DICER-independent RNAi response in a host. In this embodiment, one or more of the RNase III mutants described herein may be introduced to a host through an in vivo, in vitro, or ex vivo mechanism. In a preferred embodiment, bacteria may be transformed to heterologously express one or more RNase III mutants according to sequences according to of SEQ ID NO. 3-17, or 37-40, and 55-58. Such RNase III mutants may be introduced to a dsRNA from a pathogen, or a dsRNA that is co-expressed in said bacteria that is directed to an essential pathogen gene. The RNase III mutants may produce enhanced levels of sRNA that may further be diffused into a host and initiate an RNAi response pathway which my inhibit expression of a pathogen essential gene.

    [0302] A polynucleotide sequences encoding at least one RNase III mutant and/or a polynucleotide sequence encoding a dsRNA directed to an essential pathogen gene may be operable linked to a shared or distinct promoter. A polynucleotide sequences encoding at least one RNase III mutant and/or a polynucleotide sequence encoding a dsRNA directed to an essential pathogen gene may form an expression cassette. Further, a polynucleotide sequence encoding at least one RNase III mutant and/or a polynucleotide sequence encoding a dsRNA directed to an essential pathogen gene may form a vector that may transform a target bacteria. Methods of bacterial transformation being generally known by those of ordinary skill in the art.

    [0303] Another embodiment of the current invention includes systems, methods and compositions for the high-level generation of sRNA molecules using RNase III mutants that have enhanced catalytic activity compared to a wild type RNase III enzyme. In a preferred embodiment, RNase III mutants having enhanced catalytic activity may include an RNase III mutant having at least one of the following mutations: [0304] E38A (a glutamic acid replaced with an alanine at residue 38) according to SEQ ID NOs. 3-4; [0305] E65A (a glutamic acid replaced with an alanine at residue 65) according to SEQ ID NOs. 5-6; [0306] E38A-E65A (a glutamic acid replaced with an alanine at residue 38, and a glutamic acid replaced with an alanine at residue 65) according to SEQ ID NO. 17; [0307] E38A-R107A-R108A (a glutamic acid replaced with an alanine at residue 38, and an arginine replaced with an alanine at residue 107, and an arginine replaced with an alanine at residue 108) according to SEQ ID NOs. 7-8.

    [0308] Another embodiment of the current invention includes systems, methods and compositions for the high-level generation of sRNA molecules using RNase III mutants having enhanced stabilization of RNase III cutting patterns leading to more consistent dsRNA cutting, and increased percentages of discrete sized sRNA in a heterologous mixture of digested sRNAs compared to wildtype RNase III. In a preferred embodiment, RNase III mutants having enhanced catalytic activity may include the following RNase III mutant: [0309] E38A (a glutamic acid replaced with an alanine at residue 38) according to SEQ ID NOs. 3-4, 9-10, and 13-14; [0310] E65A (a glutamic acid replaced with an alanine at residue 65) according to SEQ ID NOs. 5-6; [0311] E38A-E65A (a glutamic acid replaced with an alanine at residue 38, and a glutamic acid replaced with an alanine at residue 65) according to SEQ ID NO. 17; [0312] E38A-R107A-R108A (a glutamic acid replaced with an alanine at residue 38, and an arginine replaced with an alanine at residue 107, and an arginine replaced with an alanine at residue 108) according to SEQ ID NOs. 7-8, 11-12, and 15-16.

    [0313] Another embodiment of the current invention includes the generation of a series of single/multiple amino acids mutants in an RNase III N-terminal catalytic domain to produce discrete-sized sRNAs, which have the potential to serve as triggers of RNA silencing. In certain embodiments, RNase III from the family Enterobacteriaceae, such as E. coli and Enterobacter, as well as from the family Bacillaceae among others, may be engineered to include one or more point mutations that improve catalytic efficiency of dsRNA cutting, as well as the production of discrete-sized sRNAs. RNase III homologs from this another families are specifically contemplated herein. Examples of additional RNase III protein sequences may include S. enterica (Uniprot ID: E7V351), P. aeruginosa (Uniprot ID: B7UYX2), C. burnetii (Uniprot ID: P51837), R. capsulatus (Uniprot ID: Q52698), S. coelicolor (Uniprot ID: Q9ZBQ7), C. jejuni (NCBI Reference Sequence: YP 001001278), H. pylori (Uniprot ID: P56118), S. aureus (Uniprot ID: P66668) and L. lactis (Uniprot ID: Q9CHD0). (Such Uniprot sequences being understood by one of ordinary skill in the art and such sequences being further incorporated herein by reference)

    [0314] Another embodiment of the current invention may include the expression of one or more RNase III mutants according to SEQ ID NOs. 3-17, or 37-40, and 55-58 in a select bacterium that may trigger RNA interference (RNAi) pathway response in an animal host. In this embodiment, for example a heterologous dsRNA directed preferably to an essential gene of a select host pathogen, may be co-expressed with one or more of the RNase III mutants described herein. In this embodiment, one or more of the RNase III mutants may generate discrete-sized sRNAs that may induce an RNAi pathway response, preferably in the animal host, and preferably in a symbiotic or endosymbiotic bacteria, such as symbiotic or endosymbiotic enteric bacteria. Exemplary animal, and in particular mammal hosts, and animal pathogens are provided in Tables 8-12, and elsewhere in the specification.

    [0315] Another embodiment of the current invention may include the expression of one or more RNase III mutants according to SEQ ID NOs. 3-17, or 37-40, and 55-58 in a select bacterium that may trigger RNA interference (RNAi) pathway response in a plant. In this embodiment, for example a heterologous dsRNA directed preferably to an essential gene of a select host pathogen, may be co-expressed with one or more of the RNase III mutants described herein. In this embodiment, one or more of the RNase III mutants may generate discrete-sized sRNAs that may induce an RNAi pathway response, preferably in the plant host and preferably in a symbiotic or endosymbiotic bacteria, such as an endophytic bacteria. Exemplary plant hosts, and plant pathogens are provided in Tables 8-12, and elsewhere in the specification.

    [0316] Another embodiment of the current invention may include the trans-kingdom delivery of sRNA molecules to a host through expression of one or more RNase III mutants according to SEQ ID NOs. 3-17, or 37-40, and 55-58 in a select symbiotic bacterium that may trigger RNA interference (RNAi) pathway response in a plant. In this embodiment, for example a heterologous dsRNA directed preferably to an essential gene of a select host pathogen, may be co-expressed with one or more of the RNase III mutants described herein in a bacterium that is a natural symbiont with the plant host. In a preferred embodiment, this natural symbiont may include one or more endophytic bacteria. In this embodiment, one or more of the RNase III mutants may generate discrete-sized sRNAs that may induce an RNAi pathway response, preferably in the plant host.

    [0317] Another embodiment of the current invention may include the trans-kingdom delivery of sRNA molecules to a host through expression of one or more RNase III mutants according to SEQ ID NOs. 3-17, or 37-40, and 55-58 in a symbiotic or endosymbiotic bacterium that may trigger RNA interference (RNAi) pathway response in an animal host. In this embodiment, for example a heterologous dsRNA directed preferably to an essential gene of a select host pathogen, may be co-expressed with one or more of the RNase III mutants described herein in a bacterium that is a natural symbiont with the plant host. In a preferred embodiment, this natural symbiont may include one or more symbiotic or endosymbiotic bacteria, and preferably an enteric bacteria. In this embodiment, one or more of the RNase III mutants may generate discrete-sized sRNAs that may induce an RNAi pathway response, preferably in the animal host.

    [0318] Another embodiment of the current invention may include the expression of one or more RNase III mutants according to SEQ ID NOs. 3-17, or 37-40, and 55-58 in a select bacterium that may produce discrete-sized sRNAs, which may trigger a prophylactic RNAi pathway response in a host. In this embodiment, for example dsRNA from a select pathogen, and preferably an essential gene of a select host pathogen may be co-expressed with one or more of the RNase III mutants described herein. In this embodiment, one or more of the RNase III mutants may generate discrete-sized sRNAs that may induce a prophylactic RNAi pathway response, preferably in the host, that may protect the host from infection by the select pathogen.

    [0319] Another embodiment of the current invention may include the expression of one or more RNase III mutants in a select bacterium that may exhibit enhanced stabilization of RNase III cutting patterns leading to more consistent dsRNA cutting and thereby produce sRNA having greater homogeneity, such that the sRNA's produced exhibit a greater consistency of size compared to wild-type or other RNase III mutants previously described in the art.

    [0320] Another embodiment of the current invention may include the expression of one or more RNase III mutants according to SEQ ID NOs. 3-17, or 37-40, and 55-58 in a select bacterium that may include a size preference for the production of discreet sized sRNA molecules. In one preferred embodiment, such discrete sized sRNA may be 26-29 nt, and/or 22-23. In one preferred embodiment, such sRNA molecules generated by one or more RNase III mutants described herein may exhibit greater homogeneity of nt size and diffusion in the host due to improved fixed-flow diffusion. With this increase diffusion, and more consistent sized sRNA molecules, a more effective and diffused RNAi response may be triggered in the host.

    [0321] Another embodiment of the current invention may include the expression of one or more RNase III mutants described herein in a select bacterium that may exhibit enhanced catalytic activity and thereby produce higher amounts of sRNA compared to wild-type or other RNase III mutants previously described in the art, and exhibit enhanced stabilization of RNase III cutting patterns leading to more consistent dsRNA cutting. In a preferred embodiment, an RNase III mutant according to SEQ ID NOs. 7-8 may be expressed in a select bacterium that may demonstrate enhanced production of discreet sized sRNA molecules of 22 to 23 nt, as well as an enhanced catalytic rate of sRNA molecule production.

    [0322] Another embodiment of the current invention may include systems, methods and compositions for the high-level production of sRNA molecules. In one preferred embodiment of the current invention may include systems, methods and compositions for the high-level production of sRNA molecules in a DICER-independent prokaryotic system. In this preferred embodiment, bacteria may be genetically modified to heterologously express one or more of the RNase III mutants, and preferably a RNase III mutant according to SEQ ID NO. 3-17, or 37-40, and 55-58 that may generate sRNA in a DICER-independent manner. The genetically modified bacteria may further co-express a target dsRNA molecule, preferably directed to an essential gene of a pathogen, pest or herbivore. These genetically modified bacteria may be grown in a fermenter, or other industrial production system known in the art. The target dsRNA molecule may be converted into sRNA molecules of a discrete size by a heterologously expressed RNase III mutant. These sRNA molecules may be generated as described above and then further isolated, while in other embodiments, the bacterium containing the sRNA molecules may be isolated or harvested for later use, such as application/administration to a plant or animal.

    [0323] Another embodiment of the invention may include compositions that include a quantity of sRNA molecules or bacteria that contain sRNA molecules generated by an RNase III mutant, and preferably a RNase III mutant according to SEQ ID NO. 3-17, or 37-40, and 55-58. Such compositions may include compositions that may be administered and/or applied to a host, such as a plant or animal host. Examples may include pharmaceutical compositions, topical compositions, encapsulated compositions, gel compositions, spray compositions and the like. Another embodiment of the invention may include the use of such sRNA molecules compositions to treat and/or prevent a pathogen caused disease condition in a host. Another embodiment of the invention may include the use of such sRNA molecules compositions to treat, prevent or kill a pest that may consume a host, preferably a plant host.

    [0324] Another embodiment of the invention may include a polynucleotide encoding one or more RNase III mutants according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15. Another embodiment of the invention may include a polynucleotide encoding one or more RNase III mutants according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15 further operably linked to a promoter. Another embodiment of the invention may include a polynucleotide encoding one or more RNase III mutants according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15 as an expression cassette. Another embodiment of the invention may include a polynucleotide encoding one or more RNase III mutants according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15 as a vector that may be used to transform a bacteria or other organism.

    [0325] Another embodiment of the invention may include a polynucleotide encoding one or more RNase III mutants according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15, and a polynucleotide encoding one or more dsRNAs directed to an essential gene in a host pathogen as generally identified in Tables 8-12. Another embodiment of the invention may include a polynucleotide encoding one or more RNase III mutants according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15, and a polynucleotide encoding one or more dsRNAs directed to an essential gene in a host pathogen wherein each sequence is operably linked to a promoter. Another embodiment of the invention may include a polynucleotide encoding one or more RNase III mutants according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15, and a polynucleotide encoding one or more dsRNAs directed to an essential gene in a host pathogen as an expression cassette. Another embodiment of the invention may include a polynucleotide encoding one or more RNase III mutants according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15, and a polynucleotide encoding one or more dsRNAs directed to an essential gene in a host pathogen as a vector that may be used to transform a bacteria or other organism.

    [0326] Another embodiment of the current invention includes systems and methods of genetically modifying a target organism, such as a target bacterium, to express a polypeptide of one or more RNase III mutants according to SEQ ID NOs. 4, 6, 8, 10, 12, 14, 16, and 17. Another embodiment of the current invention includes systems and methods of genetically modifying a target organism, such as a target bacterium, to co-express a polypeptide of one or more RNase III mutants according to SEQ ID NOs. 4, 6, 8, 10, 12, 14, 16, and 17 and a polypeptide encoding one or more dsRNAs directed to an essential gene in a host pathogen, for example as identified in Tables 8-12.

    [0327] Another embodiment of the current invention includes systems and methods of genetically modifying a target organism, such as a target bacterium, to express a polypeptide of one or more RNase III mutants according to SEQ ID NOs. 4, 6, 8, 10, 12, 14, 16, and 17. Methods of transforming a bacteria are generally known by those of ordinary skill in the art.

    [0328] Another embodiment of the invention may include an isolated polypeptide encoding one or more RNase III mutants according to SEQ ID NOs. 4, 6, 8, 10, 12, 14, 16, and 17. Another embodiment of the invention may include an isolated polynucleotide encoding one or more RNase III mutants according to SEQ ID NOs. according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15. In one prefer embodiment, a polynucleotide encoding one or more RNase III mutants according to SEQ ID NOs. according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15 may be isolated as part of a plasmid construct.

    [0329] Another embodiment may include the stable transformation of a plant or bacteria with one or more RNase III mutants according to SEQ ID NOs. 3, 5, 7, 9, 11, 13, and 15. Another embodiment may include the stable transformation of a plant or bacteria that expresses one or more RNase III mutants according to SEQ ID NOs. 4, 6, 8, 10, 12, 14, 16, and 17.

    [0330] Another embodiment of the invention may include the generation of a series of single/multiple amino acids mutants in an RNase III, wherein the RNase III is a bacterial RNase III. Another embodiment of the invention may include the generation of a series of single/multiple amino acids mutants in an RNase III from E. coli, preferably according to SEQ ID NOs.3-8, and 17. In one embodiment, an RNase III from E. coli may be according to polynucleotide sequence SEQ ID NO. 1, and/or amino acid sequence SEQ ID NO. 2.

    [0331] Another embodiment of the invention may include the generation of a series of single/multiple amino acids mutants in an RNase III from Enterobacteriaceae, preferably according to SEQ ID NOs. 9-12. Another embodiment of the invention may include the generation of a series of single/multiple amino acids mutants in an RNase III from Enterobacter, preferably according to SEQ ID NOs. 13-16. Another embodiment of the invention may include the generation of a series of single/multiple amino acids mutants in an RNase III, wherein the RNase III is a homolog of an RNase III described herein. Another embodiment of the invention may include the generation of a series of single/multiple amino acids mutants in an RNase III, wherein the RNase III is an ortholog of an RNase III described herein.

    [0332] Another embodiment of the current invention may include the generation of an E38A RNase III mutant. Another embodiment of the current invention may include the transformation and/or expression of an E38A RNase III mutant in bacteria. Another embodiment of the current invention may include the transformation and/or expression of an E38A RNase III mutant in bacteria that is symbiotic or endosymbiotic with a target host. Another embodiment of the current invention may include the transformation and/or expression of a an E38A RNase III mutant in bacteria that is symbiotic or endosymbiotic with a target host, wherein the RNase III mutant generates sRNA that are delivered to the target host and induce an RNAi pathway response. Another embodiment of the current invention may include the co-expression in a bacterium of an E38A RNase III mutant and a dsRNA directed to an essential pathogen gene in a target host.

    [0333] Another embodiment of the current invention may include the generation of an E65A RNase III mutant. Another embodiment of the current invention may include the transformation and/or expression of an E65A RNase III mutant in bacteria. Another embodiment of the current invention may include the transformation and/or expression of an E65A RNase III mutant in bacteria that is symbiotic or endosymbiotic with a target host. Another embodiment of the current invention may include the transformation and/or expression of a an E65A RNase III mutant in bacteria that is symbiotic or endosymbiotic with a target host, wherein the RNase III mutant generates sRNA that are delivered to the target host and induce an RNAi pathway response. Another embodiment of the current invention may include the co-expression in a bacterium of an E65A RNase III mutant and a dsRNA directed to an essential pathogen gene in a target host.

    [0334] Another embodiment of the current invention may include the generation of an E38A-E65A RNase III mutant. Another embodiment of the current invention may include the transformation and/or expression of an E38A-E65A RNase III mutant in bacteria. Another embodiment of the current invention may include the transformation and/or expression of an E38A-E65A RNase III mutant in bacteria that is symbiotic or endosymbiotic with a target host. Another embodiment of the current invention may include the transformation and/or expression of a an E38A-E65A RNase III mutant in bacteria that is symbiotic or endosymbiotic with a target host, wherein the RNase III mutant generates sRNA that are delivered to the target host and induce an RNAi pathway response. Another embodiment of the current invention may include the co-expression in a bacterium of an E38A-E65A RNase III mutant and a dsRNA directed to an essential pathogen gene in a target host.

    [0335] Another embodiment of the current invention may include the generation of an E38A-R107A-R108A RNase III mutant. Another embodiment of the current invention may include the transformation and/or expression of an E38A-R107A-R108A RNase III mutant in a bacteria. Another embodiment of the current invention may include the transformation and/or expression of an E38A-R107A-R108A RNase III mutant in bacteria that is symbiotic or endosymbiotic with a target host. Another embodiment of the current invention may include the transformation and/or expression of a an E38A-R107A-R108A RNase III mutant in bacteria that is symbiotic or endosymbiotic with a target host, wherein the RNase III mutant generates sRNA that are delivered to the target host and induce an RNAi pathway response. Another embodiment of the current invention may include the co-expression in a bacterium of an E38A-R107A-R108A RNase III mutant and a dsRNA directed to an essential pathogen gene in a target host.

    [0336] Another embodiment of the current invention may include the generation of an E38A RNase III mutant having a size preference for the generation of 26 and 29 nt sRNAs. Another embodiment of the current invention may include the generation of an E38A RNase III mutant having improved catalytic efficiency. Another embodiment of the current invention may include the generation of an E38A RNase III mutant according to SEQ ID NOs. 3-4, 13-14, and 9-10.

    [0337] Another embodiment of the current invention may include the generation of an E65A RNase III mutant having a size preference for the generation of 26 and 29 nt sRNAs. Another embodiment of the current invention may include the generation of an E65A RNase III mutant having improved catalytic efficiency. Another embodiment of the current invention may include the generation of an E65A RNase III mutant according to SEQ ID NO. 5-6.

    [0338] Another embodiment of the current invention may include the generation of an E38A-E65A RNase III mutant having a size preference for the generation of 26 and 29 nt sRNAs. Another embodiment of the current invention may include the generation of an E38A-E65A RNase III mutant having improved catalytic efficiency. Another embodiment of the current invention may include the generation of an E65A RNase III mutant according to SEQ ID NO. 17.

    [0339] Another embodiment of the current invention may include the generation of an E38A-R107A-R108A RNase III mutant having a size preference for the generation of 22 and 23 nt sRNAs. Another embodiment of the current invention may include the generation of an E38A-R107A-R108A RNase III mutant having improved catalytic efficiency and enhanced dsRNA cutting specificity for 22 and 23 nt sRNAs. Another embodiment of the current invention may include the generation of an E65A RNase III mutant according to SEQ ID NO. 7-8, 11-12, and 15-16.

    [0340] Another embodiment of the current invention may include the generation of one or more RNase III mutants that may be expressed in bacteria and generate sRNA that may be further isolated. In one preferred embodiment, the current invention may include the generation of RNase III mutants that may be expressed in bacteria and generate sRNA according to SEQ ID NOs. 3-17, or 37-40, and 55-58.

    [0341] Another embodiment of the current invention may include the generation of one or more RNase III mutants that may be expressed in bacteria configured to deliver sRNA to a host. In one preferred embodiment, the current invention may include the generation of RNase III mutants according to SEQ ID NOs. 3-17, or 37-40, and 55-58 that may be expressed in bacteria configured to deliver sRNA to a host and initiate a DICER-independent RNAi pathway response.

    [0342] Another embodiment of the current invention may include the generation of one or more RNase III mutants according to SEQ ID NOs. 3-17, or 37-40, and 55-58 that may be co-expressed with a dsRNA directed to an essential pathogen gene, preferably a symbiotic and/or endosymbiotic bacteria to the host. In this embodiment, the RNase III mutants that may generate sRNA from the co-expressed dsRNA and to deliver the sRNA to a host initiating a RNAi pathway response.

    [0343] Another embodiment of the current invention may include the generation of one or more RNase III mutants according to SEQ ID NOs. 3-17, or 37-40, and 55-58 that may be co-expressed with a dsRNA directed to an essential pest gene, preferably a symbiotic and/or endosymbiotic bacteria to the host. In this embodiment, the RNase III mutants that may generate sRNA from the co-expressed dsRNA and to deliver the sRNA to a host initiating a RNAi pathway response in pest consuming the host, preferably a plant.

    [0344] In another embodiment, the present inventors may generate a RNase III mutant that is integrated into a bacterial chromosome. In a preferred embodiment, an RNAase III mutant may include, but not be limited to: [0345] E38A (a glutamic acid replaced with an alanine at residue 38) according to SEQ ID NOs. 3-4, 9-10, and 13-14; [0346] E65A (a glutamic acid replaced with an alanine at residue 65) according to SEQ ID NOs. 5-6; [0347] E38A-E65A (a glutamic acid replaced with an alanine at residue 38, and a glutamic acid replaced with an alanine at residue 65) according to SEQ ID NO. 17; [0348] E38A-R107A-R108A (a glutamic acid replaced with an alanine at residue 38, and an arginine replaced with an alanine at residue 107, and an arginine replaced with an alanine at residue 108) according to SEQ ID NOs. 7-8, 11-12, and 15-16.

    [0349] In a preferred embodiment, an RNAase III mutant according to SEQ ID NOs. 3-17, or 37-40, and 55-58 may be integrated into a bacterial chromosome and expressed.

    [0350] In further aspects, the present invention includes methods of administering a therapeutically effective amount of one or more genetically modified bacteria expressing a heterologous RNase III mutant and a dsRNA directed to an essential pathogen gene as generally described above.

    [0351] The following definitions are provided to aid the reader in understanding the various aspects of the present disclosure. Unless defined otherwise, all technical and scientific terms used herein have the same meaning as commonly understood by those of ordinary skill in the art to which the disclosure pertains.

    [0352] As used herein and in the appended claims, the singular forms “a”, “an”, and “the” include plural referents unless the context clearly dictates otherwise. Thus, for example, reference to “a plant” includes a plurality of such plants; reference to “a cell” includes one or more cells and equivalents thereof known to those skilled in the art, and so forth. Similarly, the word “or” is intended to include “and” unless the context clearly indicates otherwise. Hence “comprising A or B” means including A, or B, or A and B. Furthermore, the use of the term “including”, as well as other related forms, such as “includes” and “included”, is not limiting.

    [0353] The term “about” as used herein is a flexible word with a meaning similar to “approximately” or “nearly”. The term “about” indicates that exactitude is not claimed, but rather a contemplated variation. Thus, as used herein, the term “about” means within 1 or 2 standard deviations from the specifically recited value, or ±a range of up to 20%, up to 15%, up to 10%, up to 5%, or up to 4%, 3%, 2%, or 1% compared to the specifically recited value.

    [0354] The term “comprising” as used in a claim herein is open-ended, and means that the claim must have all the features specifically recited therein, but that there is no bar on additional features that are not recited being present as well. The term “comprising” leaves the claim open for the inclusion of unspecified ingredients even in major amounts. The term “consisting essentially of” in a claim means that the invention necessarily includes the listed ingredients, and is open to unlisted ingredients that do not materially affect the basic and novel properties of the invention. A “consisting essentially of” claim occupies a middle ground between closed claims that are written in a closed “consisting of” format and fully open claims that are drafted in a “comprising’ format”. These terms can be used interchangeably herein if, and when, this may become necessary. Furthermore, the use of the term “including”, as well as other related forms, such as “includes” and “included”, is not limiting. Notably, where the specification or other parts of this application refer to a polynucleotide sequence, it may also refer to the corresponding protein sequence and vice versa.

    [0355] The term “derived” means an RNase III that was mutated to generate an RNase III mutant. The term “fed” means introducing a bacteria expressing a RNase III mutant to an animal, for example directly, or through a feed infused with the bacteria or other cell.

    [0356] “RNase III” refers to a naturally occurring enzyme or its recombinant form. The RNase III family of dsRNA-specific endonucleases is characterized by the presence of a highly conserved 9 amino acid stretch in their catalytic center known as the RNaseIII signature motif. Mutants and derivatives are included in the definition. The utility of bacterial RNase III described herein to achieve silencing in mammalian cells further supports the use of RNases from eukaryotes, prokaryotes viruses or archaea in the present embodiments based on the presence of common characteristic consensus sequences. The designations for the mutants are assigned by an amino acid position in a particular RNaseIII isolate. These amino acid positions may vary between RNase III enzymes from different sources. For example, E38 in E. coli corresponds to E37 in Aquifex aeolicus. The positions E38 in E. coli and E37 in A. aeolicus correspond to the first amino acid position of the consensus sequence described above and determined by aligning RNaseIII amino acid sequences from the public databases by their consensus sequences. Embodiments of the invention are not intended to be limited to the actual number designation. Preferred embodiments refer to relative position of the amino acid in the RNaseIII consensus sequence(s). In particular, the invention includes residues 38, 65, 107 and 108 and their corresponding residues across various homologous bacterial RNase III proteins, or homologs.

    [0357] Mutations in the RNaseIII refer to any of point mutations, additions, deletions (though preferably not in the cleavage domain), and rearrangements (preferably in the domain linking regions). Mutations may be at a single site or at multiple sites in the RNaseIII protein. Mutations can be generated by standard techniques including random mutagenesis, targeted genetics and other methods known by those of ordinary skill in the art.

    [0358] According to the present invention “sRNA” is small RNA, in particular RNA of a length of 200 nucleotides or less that is not translated into a protein. sRNA may be RNA molecules digested by one or more of the RNase III mutants described herein. sRNA may include siRNA mRNA, or even dsRNA molecules that may be generated by or initiate an RNAi pathway response which may result in the downregulation of a target gene. “RNAi” refers to gene downregulation or inhibition that is induced by the introduction of a double-stranded RNA molecule.

    [0359] In still other embodiments of the invention, inhibition of the expression of one or more pathogen gene products by RNAi may be obtained through a dsRNA-mediated RNAi action and/or a form of dsRNA known as a hairpin RNA (hpRNA) interference or intron-containing hairpin RNA (ihpRNA) interference. For hpRNA interference, the expression cassette is designed to express an RNA molecule that hybridizes with itself to form a hairpin structure that comprises a single-stranded loop region and a base-paired stem. The base-paired stem region comprises a sense sequence corresponding to all or part of the endogenous messenger RNA encoding the gene product whose expression is to be inhibited, in this case, a pathogen essential gene described herein, and an antisense sequence that is fully or partially complementary to the sense sequence. Alternatively, the base-paired stem region may correspond to a portion of a promoter sequence controlling expression of the gene encoding the target polypeptide to be inhibited. Thus, the base-paired stem region of the molecule generally determines the specificity of the RNA interference. HpRNA molecules are highly efficient at inhibiting the expression of endogenous genes, and the RNA interference they induce is inherited by subsequent generations of plants. See, for example, Chuang and Meyerowitz (2000) Proc. Natl. Acad. Sci. USA 97:4985-4990; Stoutjesdijk et al. (2002) Plant Physiol. 129:1723-1731; and Waterhouse and Helliwell (2003) Nat. Rev. Genet. 4:29-38. Methods for using hpRNA interference to inhibit or silence the expression of genes are described, for example, in Chuang and Meyerowitz (2000) Proc. Natl. Acad. Sci. USA 97:4985-4990; Stoutjesdijk et al. (2002) Plant Physiol. 129:1723-1731; Waterhouse and Helliwell (2003) Nat. Rev. Genet. 4:29-38; Pandolfini et al. BMC Biotechnology 3:7, and U.S. Patent Publication No. 20030175965; each of which is herein incorporated by reference. A transient assay for the efficiency of hpRNA constructs to silence gene expression in vivo has been described by Panstruga et al. (2003) Mol. Biol. Rep. 30:135-140, herein incorporated by reference.

    [0360] For ihpRNA, the interfering molecules have the same general structure as for hpRNA, but the RNA molecule additionally comprises an intron that is capable of being spliced in the cell in which the ihpRNA is expressed. The use of an intron minimizes the size of the loop in the hairpin RNA molecule following splicing, and this increases the efficiency of interference. See, for example, Smith et al. (2000) Nature 407:319-320. In fact, Smith et al. show 100% suppression of endogenous gene expression using ihpRNA-mediated interference. Methods for using ihpRNA interference to inhibit the expression of endogenous plant genes are described, for example, in Smith et al. (2000) Nature 407:319-320; Wesley et al. (2001) Plant J 27:581-590; Wang and Waterhouse (2001) Curr. Opin. Plant Biol. 5:146-150; Waterhouse and Helliwell (2003) Nat. Rev. Genet. 4:29-38; Helliwell and Waterhouse (2003) Methods 30:289-295, and U.S. Patent Publication No. 20030180945, each of which is herein incorporated by reference.

    [0361] The term “gene” or “gene sequence” refers to a coding region operably joined to appropriate regulatory sequences capable of regulating the expression of the gene product (e.g., a polypeptide or a functional RNA) in some manner. A gene includes untranslated regulatory regions of DNA (e.g., promoters, enhancers, repressors, etc.) preceding (up-stream) and following (down-stream) the coding region (open reading frame, ORF) as well as, where applicable, intervening sequences (i.e., introns) between individual coding regions (i.e., exons). The term “structural gene” as used herein is intended to mean a DNA sequence that is transcribed into mRNA which is then translated into a sequence of amino acids characteristic of a specific polypeptide.

    [0362] As used herein, “inhibit, “inhibition,” “suppress,” “downregulate” or “silencing” refers to partial or complete loss-of-function through targeted inhibition of gene expression in a cell and may also be referred to as “knock down,” preferably through an RNAi pathway response. Depending on the circumstances and the biological problem to be addressed, it may be preferable to partially reduce gene expression. Alternatively, it might be desirable to reduce gene expression as much as possible. The extent of silencing may be determined by any method known in the art, some of which are summarized in International Publication No. WO 99/32619, incorporated herein by reference. As used herein, ““inhibit, “inhibition, ““suppress,” “downregulate” or “silencing” of the level or activity of an agent, such as, for example, a preRNA, mRNA, rRNA, tRNA, snoRNA, snRNA expressed by the target gene, and/or of the protein product encoded by it, means that the amount is reduced by 10% or more, for example, 20% or more, preferably 30% or more, more preferably 50% or more, even more preferably 70% or more, most preferably 80% or more, for example, 90%, relative to a cell or organism lacking a dsRNA molecule of the disclosure.

    [0363] “Large double-stranded RNA” refers to any dsRNA or hairpin having a double-stranded region greater than about 40 base pairs (bp) for example, larger than 100 bp, or more, particularly larger than 300 bp. The sequence of a large dsRNA may represent one or more segments of one or more mRNAs or the entire mRNAs. The maximum size of the large dsRNA is not limited herein. The dsRNA may include modified bases where the modification may be to the phosphate sugar backbone or to the nucleotide. Such modifications may include a nitrogen or sulfur heteroatom or any other modification known in the art. The dsRNA may be made enzymatically, by recombinant techniques, and/or by chemical synthesis or using commercial kits such as MEGASCRIPT® (Ambion, Austin, Tex.) and methods known in the art. An embodiment of the invention utilizes HiScribe™ (New England Biolabs, Inc., Beverly, Mass.) for making large dsRNA. Other methods for making and storing large dsRNA are described in International Publication No. WO 99/32619. The double-stranded structure may be formed by a self-complementary RNA strand such as occurs for a hairpin or a micro RNA, or by annealing of two distinct complementary RNA strands.

    [0364] As used herein a “wild type” means a cell or organism that does not contain the heterologous recombinant DNA that expressed a protein or element that imparts an enhanced trait as described herein.

    [0365] “Expression” or “expressing” refers to production of a functional product, such as, the generation of an RNA transcript from an introduced construct, an endogenous DNA sequence, or a stably incorporated heterologous DNA sequence. A nucleotide encoding sequence may comprise intervening sequence (e.g., intrans) or may lack such intervening non-translated sequences (e.g., as in cDNA). Expressed genes include those that are transcribed into mRNA and then translated into protein and those that are transcribed into RNA but not translated (for example, siRNA, transfer RNA, and ribosomal RNA). The term may also refer to a polypeptide produced from an mRNA generated from any of the above DNA precursors. Thus, expression of a nucleic acid fragment, such as a gene or a promoter region of a gene, may refer to transcription of the nucleic acid fragment (e.g., transcription resulting in mRNA or other functional RNA) and/or translation of RNA into a precursor or mature protein (polypeptide), or both.

    [0366] An “expression cassette or “expression vector” or “vector” refers to a nucleic acid construct, which when introduced into a host cell, results in transcription and/or translation of a RNA or polypeptide, respectively. More specifically, the term “vector” refers to some means by which DNA, RNA, a protein, or polypeptide can be introduced into a host. The polynucleotides, protein, and polypeptide which are to be introduced into a host can be therapeutic or prophylactic in nature; can encode or be an antigen; can be regulatory in nature, etc. There are various types of vectors including virus, plasmid, bacteriophages, cosmids, and bacteria. Again, more specifically, “expression vector” is nucleic acid capable of replicating in a selected host cell or organism. An expression vector can replicate as an autonomous structure, or alternatively can integrate, in whole or in part, into the host cell chromosomes or the nucleic acids of an organelle, or it is used as a shuttle for delivering foreign DNA to cells, and thus replicate along with the host cell genome. Thus, an expression vector are polynucleotides capable of replicating in a selected host cell, organelle, or organism, e.g., a plasmid, virus, artificial chromosome, nucleic acid fragment, and for which certain genes on the expression vector (including genes of interest) are transcribed and translated into a polypeptide or protein within the cell, organelle or organism; or any suitable construct known in the art, which comprises an “expression cassette.” In contrast, as described in the examples herein, a “cassette” is a polynucleotide containing a section of an expression vector of this invention. The use of the cassettes assists in the assembly of the expression vectors. An expression vector is a replicon, such as plasmid, phage, virus, chimeric virus, or cosmid, and which contains the desired polynucleotide sequence operably linked to the expression control sequence(s). A polynucleotide sequence is operably linked to an expression control sequence(s) (e.g., a promoter and, optionally, an enhancer) when the expression control sequence controls and regulates the transcription and/or translation of that polynucleotide sequence.

    [0367] The term “genome” encompasses not only chromosomal DNA found within the nucleus, but organelle DNA found within subcellular components (e.g., mitochondrial, plastid) of the cell. As used herein, the term “genome” refers to the nuclear genome unless indicated otherwise.

    [0368] The term “heterologous” refers to a nucleic acid fragment or protein that is foreign to its surroundings. In the context of a nucleic acid fragment, this is typically accomplished by introducing such fragment, derived from one source, into a different host. Heterologous nucleic acid fragments, such as coding sequences that have been inserted into a host organism, are not normally found in the genetic complement of the host organism. As used herein, the term “heterologous” also refers to a nucleic acid fragment derived from the same organism, but which is located in a different, e.g., non-native, location within the genome of this organism. Thus, the organism can have more than the usual number of copy(ies) of such fragment located in its(their) normal position within the genome and in addition, in the case of plant cells, within different genomes within a cell, for example in the nuclear genome and within a plastid or mitochondrial genome as well. A nucleic acid fragment that is heterologous with respect to an organism into which it has been inserted or transferred is sometimes referred to as a “transgene.”

    [0369] “Host cell” means a cell which contains an expression vector and supports the replication and/or expression of that vector. The term “introduced” means providing a nucleic acid (e.g., an expression construct) or protein into a cell. “Introduced” includes reference to the incorporation of a nucleic acid into a eukaryotic or prokaryotic cell where the nucleic acid may be incorporated into the genome of the cell, and includes reference to the transient provision of a nucleic acid or protein to the cell. “Introduced” includes reference to stable or transient transformation methods, as well as sexually crossing. Thus, “introduced” in the context of inserting a nucleic acid fragment (e.g., a recombinant DNA construct/expression construct) into a cell, can mean “transfection” or “transformation” or “transduction”, and includes reference to the incorporation of a nucleic acid fragment into a eukaryotic or prokaryotic cell where the nucleic acid fragment may be incorporated into the genome of the cell (e.g., chromosome, plasmid, plastid, or mitochondrial DNA), converted into an autonomous replicon, or transiently expressed (e.g., transfected mRNA).

    [0370] As used herein, “nucleic acid” or “nucleotide sequence” means a polynucleotide (or oligonucleotide), including single or double-stranded polymers of deoxyribonucleotides or ribonucleotide bases, and unless otherwise indicated, encompasses naturally occurring and synthetic nucleotide analogues having the essential nature of natural nucleotides in that they hybridize to complementary single stranded nucleic acids in a manner similar to naturally occurring nucleotides. Nucleic acids may also include fragments and modified nucleotide sequences. Nucleic acids disclosed herein can either be naturally occurring, for example genomic nucleic acids, or isolated, purified, nongenomic nucleic acids, including synthetically produced nucleic acid sequences such as those made by solid phase chemical oligonucleotide synthesis, enzymatic synthesis, or by recombinant methods, including for example, cDNA, codon-optimized sequences for efficient expression in different transgenic plants reflecting the pattern of codon usage in such plants, nucleotide sequences that differ from the nucleotide sequences disclosed herein due to the degeneracy of the genetic code but that still encode the protein(s) of interest disclosed herein, nucleotide sequences encoding the presently disclosed protein(s) comprising conservative (or non-conservative) amino acid substitutions that do not adversely affect their normal activity, PCR-amplified nucleotide sequences, and other non-genomic forms of nucleotide sequences familiar to those of ordinary skill in the art.

    [0371] “Nucleic acid construct” or “construct” refers to an isolated polynucleotide which can be introduced into a host cell, for example a plasmid. This construct may comprise any combination of deoxyribonucleotides, ribonucleotides, and/or modified nucleotides. This construct may comprise an expression cassette that can be introduced into and expressed in a host cell.

    [0372] “Operably linked” refers to a functional arrangement of elements. A first nucleic acid sequence is operably linked with a second nucleic acid sequence when the first nucleic acid sequence is placed in a functional relationship with the second nucleic acid sequence. For instance, a promoter is operably linked to a coding sequence if the promoter effects the transcription or expression of the coding sequence. The control elements need not be contiguous with the coding sequence, so long as they function to direct the expression thereof. Thus, for example, intervening untranslated yet transcribed sequences can be present between a promoter and the coding sequence and the promoter can still be considered “operably linked” to the coding sequence.

    [0373] The terms “peptide”, “polypeptide”, and “protein” are used to refer to polymers of amino acid residues. These terms are specifically intended to cover naturally occurring biomolecules, as well as those that are recombinantly or synthetically produced, for example by solid phase synthesis.

    [0374] The term “promoter” or “regulatory element” refers to a region or nucleic acid sequence located upstream or downstream from the start of transcription and which is involved in recognition and binding of RNA polymerase and/or other proteins to initiate transcription of RNA. Promoters need not be of plant or algal origin. For example, promoters derived from plant viruses, such as the CaMV35S promoter, or from other organisms, can be used in variations of the embodiments discussed herein. Promoters useful in the present methods include, for example, constitutive, strong, weak, tissue-specific, cell-type specific, seed-specific, inducible, repressible, and developmentally regulated promoters. Examples of suitable promoters for gene suppressing cassettes include, but are not limited to, T7 promoter, bla promotor, U6 promoter, pol II promoter, Ell promoter, and CMV promoter and the like.

    [0375] A “cell type-specific” promoter primarily drives expression in certain cell types in one or more organs. An “inducible” promoter may be a promoter which may be under environmental control or induced by a secondary molecule or compound Tissue-specific, tissue-preferred, cell type specific, and inducible promoters constitute the class of “non-constitutive” promoters. A “constitutive” promoter is a promoter which may be active under most environmental conditions or in most cell or tissue types.

    [0376] As used herein, the term “transformation” or “genetically modified” refers to the transfer of one or more nucleic acid molecule(s) into a cell. A microorganism is “transformed” or “genetically modified” by a nucleic acid molecule transduced into the bacteria when the nucleic acid molecule becomes stably replicated by the bacteria. As used herein, the term “transformation” or “genetically modified” encompasses all techniques by which a nucleic acid molecule can be introduced into, such as a bacterium.

    [0377] As used herein, a “genetically modified plant or “transgenic plant” is one whose genome has been altered by the incorporation of exogenous genetic material, e.g. by transformation as described herein. The term “transgenic plant” is used to refer to the plant produced from an original transformation event, or progeny from later generations or crosses of a transgenic plant so long as the progeny contains the exogenous genetic material in its genome. By “exogenous” is meant that a nucleic acid molecule, for example, a recombinant DNA, originates from outside the plant into which it is introduced. An exogenous nucleic acid molecule may comprise naturally or non-naturally occurring DNA, and may be derived from the same or a different plant species than that into which it is introduced.

    [0378] “Stable transformation” is intended to mean that the nucleotide construct introduced into a host and integrates into the genome of the plant and is capable of being inherited by the progeny thereof. The nucleic acid molecule can be transiently expressed or non-stably maintained in a functional form in the cell for less than three months i.e. is transiently expressed.

    [0379] The terms “plant” or “plants” that can be used in the present methods broadly include the classes of higher and lower plants amenable to transformation techniques, including angiosperms (monocotyledonous and dicotyledonous plants), gymnosperms, ferns, and unicellular and multicellular algae. The term “plant” also includes plants which have been modified by breeding, mutagenesis, or genetic engineering (transgenic and non-transgenic plants). It includes plants of a variety of ploidy levels, including aneuploid, polyploid, diploid, haploid, and hemizygous. The plant may be in any form including suspension cultures, embryos, meristematic regions, callus tissue, gametophytes, sporophytes, pollen, microspores, whole plants, shoot vegetative organs/structures (e.g. leaves, stems and tubers), roots, flowers and floral organs/structures, seed (including embryo, endosperm, and seed coat) and fruit, plant tissue (e.g. vascular tissue, ground tissue, and the like) and cells, and progeny of same.

    [0380] The term “probiotic” refers to a microorganism, such as bacteria, that may colonize a host for a sufficient length of time to delver a therapeutic or effective amount of an interfering RNA molecule. A probiotic may include endosymbiotic bacteria, or naturally occurring flora that may permanently to temporarily colonize an animal, such as an aquatic organism. Probiotic organisms may also include algae, and fungi, such as yeast.

    [0381] The invention encompasses isolated or substantially purified RNase III mutant polynucleotides or amino acid compositions. An “isolated” or “purified” RNase III mutant polynucleotide or protein, or biologically active portion thereof, is substantially or essentially free from components that normally accompany or interact with the RNase III mutant polynucleotide or protein as found in its naturally occurring environment. Thus, an isolated or purified polynucleotide or protein is substantially free of other cellular material, or culture medium when produced by recombinant techniques, or substantially free of chemical precursors or other chemicals when chemically synthesized. Optimally, an “isolated” polynucleotide is free of sequences (optimally protein encoding sequences) that naturally flank the polynucleotide (i.e., sequences located at the 5′ and 3′ ends of the polynucleotide) in the genomic DNA of the organism from which the polynucleotide is derived.

    [0382] A “variant,” or “isoform,” or “protein variant” is a member of a set of similar proteins that perform the same or similar biological roles. For example, fragments and variants of the disclosed RNase III polynucleotides and amino acid sequences encoded thereby are also encompassed by the present invention. By “fragment” is intended a portion of the polynucleotide or a portion of the amino acid sequence. For polynucleotides, a variant comprises a polynucleotide having deletions (i.e., truncations) at the 5′ and/or 3′ end; deletion and/or addition of one or more nucleotides at one or more internal sites in the native polynucleotide; and/or substitution of one or more nucleotides at one or more sites in the native polynucleotide. As used herein, a “native” or “wildtype” polynucleotide or polypeptide comprises a naturally occurring nucleotide sequence or amino acid sequence, respectively. Generally, variants of a particular RNase III disclosed herein will have at least about 75%, 80%, 85%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99% or more sequence identity to that particular polynucleotide as determined by sequence alignment programs and parameters as described elsewhere herein.

    [0383] The compositions disclosed herein also comprise synthetic oligonucleotides or nucleotide sequences encoding RNase III mutant sequences. A synthetic sequence is one that is produced or reproduced in a laboratory setting. While the nucleotide sequence may have an altered nucleotide sequence relative to the parent sequence, the synthetic sequence may be identical to the naturally occurring sequence. In both instances, however, the structure of the synthetic sequence is altered or different from that found in the sequence that is directly isolated from its natural setting.

    [0384] As used herein, the phrase “host” refers to an organism, such as a plant or animal, carrying a disease-causing pathogen, an organism susceptible to a disease-causing pathogen, an organism population where members are carrying a disease-causing pathogen, or an organism population where members are susceptible to a disease-causing pathogen. These include hosts listed in tables 8-12, and elsewhere. In one embodiment a target host may be a aquatic organism, and preferably an organism grown in aquaculture. The term “aquaculture” as used herein includes the cultivation of aquatic organisms under controlled conditions. The term “aquatic organism” and/or “aquatic animal” as used herein include organisms grown in water, either fresh or saltwater. Aquatic organisms/animals includes vertebrates, invertebrates, arthropods, fish, mollusks, including, shrimp (e.g., penaeid shrimp, Penaeus esculentu, Penaeus setiferus, Penaeus stylirostris, Penaeus occidentalis, Penaeus japonicus, Penaeus vannamei, Penaeus monodon, Penaeus chinensis, Penaeus aztecus, Penaeus duorarum, Penaeus indicus, and Penaeus merguiensis, Penaeus californiensis, Penaeus semisulcatus, Penaeus monodon, brine shrimp, freshwater shrimp, etc), crabs, oysters, scallop, prawn clams, cartilaginous fish (e.g., sea bream, trout, bass, striped bass, tilapia, catfish, salmonids, carp, catfish, yellowtail, carp zebrafish, red drum, etc), crustaceans, among others. Shrimp include shrimp raised in aquaculture as well. Example pathogens affecting aquatic organisms may include white spot syndrome (WSS)

    [0385] As used herein, “pathogen” refers to a disease causing agent. These include the pathogens included in tables 8-12, and elsewhere.

    [0386] “Target” or “essential gene” refers to any gene or mRNA of interest. Indeed any of the genes previously identified by genetics or by sequencing may represent a target. Target genes or mRNA may include developmental genes and regulatory genes as well as metabolic or structural genes or genes encoding enzymes. The target gene may be expressed in those cells in which a phenotype is being investigated or in an organism in a manner that directly or indirectly impacts a phenotypic characteristic. The target gene may be endogenous or exogenous. An “essential gene,” for example may be a gene necessary for survival, replication or pathogenicity in a pathogen. Such cells include any cell in the body of an adult or embryonic animal or plant including gamete or any isolated cell such as occurs in an immortal cell line or primary cell culture.

    [0387] Moreover, the terms “enhance”, “enhanced”, “increase”, “increased” or “improved” generally refer to a statistically significant increase, for example in a trait, phenotype or catalytic rate. For the avoidance of doubt, these terms generally refer to about a 5% increase in a given parameter or value, about a 10% increase, about a 15% increase, about a 20% increase, about a 25% increase, about a 30% increase, about a 35% increase, about a 40% increase, about a 45% increase, about a 50% increase, about a 55% increase, about a 60% increase, about a 65% increase, about 70% increase, about a 75% increase, about an 80% increase, about an 85% increase, about a 90% increase, about a 95% increase, about a 100% increase, or more over the control value. These terms also encompass ranges consisting of any lower indicated value to any higher indicated value, for example “from about 5% to about 50%”, etc.

    [0388] Unless otherwise stated, nucleic acid sequences in the text of this specification are given, when read from left to right, in the 5′ to 3′ direction. Nucleic acid sequences may be provided as DNA or as RNA, as specified; disclosure of one necessarily defines the other, as is known to one of ordinary skill in the art and is understood as included in embodiments where it would be appropriate. Nucleotides may be referred to by their commonly accepted single-letter codes. Unless otherwise indicated, amino acid sequences are written left to right in amino to carboxyl orientation, respectively. Amino acids may be referred to herein by either their commonly known three letter symbols or by the one-letter symbols as generally understood by those skilled in the relevant art.

    [0389] Regarding disclosed ranges, the endpoints of all ranges directed to the same component or property are inclusive and independently combinable (e.g., ranges of “about 25%, or, more, about 5% to about 20 wt. %,” is inclusive of the endpoints and all intermediate values of the ranges of “about 5% to about 25%,” etc.). Numeric ranges recited with the specification are inclusive of the numbers defining the range and include each integer within the defined range.

    [0390] Notably, all peptides disclosed in specifically encompass peptides having conservative amino acid substitutions. As used herein, “conservative amino acid substitutions” means the manifestation that certain amino acids can be substituted for other amino acids in a protein structure without appreciable loss of biochemical or biological activity. Since it is the interactive capacity and nature of a protein that defines that protein's biological functional activity, certain amino acid sequence substitutions can be made in a protein sequence, and, of course, the underlying DNA coding sequence, and nevertheless obtain a protein with like properties. Thus, various changes can be made in the amino acid sequences disclosed herein, or in the corresponding DNA sequences that encode these amino acid sequences, without appreciable loss of their biological utility or activity.

    [0391] Examples of amino acid groups defined in this manner include: a “charged polar group,” consisting of glutamic acid (Glu), aspartic acid (Asp), asparagine (Asn), glutamine (Gln), lysine (Lys), arginine (Arg) and histidine (His); an “aromatic, or cyclic group,” consisting of proline (Pro), phenylalanine (Phe), tyrosine (Tyr) and tryptophan (Trp); and an “aliphatic group” consisting of glycine (Gly), alanine (Ala), valine (Val), leucine (Leu), isoleucine (Ile), methionine (Met), serine (Ser), threonine (Thr) and cysteine (Cys).

    [0392] Within each group, subgroups can also be identified, for example, the group of charged polar amino acids can be sub-divided into the sub-groups consisting of the “positively-charged sub-group,” consisting of Lys, Arg and His; the negatively-charged sub-group,” consisting of Glu and Asp, and the “polar sub-group” consisting of Asn and Gin. The aromatic or cyclic group can be sub-divided into the sub-groups consisting of the “nitrogen ring sub-group,” consisting of Pro, His and Trp; and the “phenyl sub-group” consisting of Phe and Tyr. The aliphatic group can be sub-divided into the sub-groups consisting of the “large aliphatic non-polar sub-group,” consisting of Val, Leu and Ile; the “aliphatic slightly-polar sub-group,” consisting of Met, Ser, Thr and Cys; and the “small-residue sub-group,” consisting of Gly and Ala. Examples of conservative mutations include substitutions of amino acids within the sub-groups above, for example, Lys for Arg and vice versa such that a positive charge can be maintained; Glu for Asp and vice versa such that a negative charge can be maintained; Ser for Thr such that a free —OH can be maintained; and Gin for Asn such that a free —NH2 can be maintained.

    [0393] Proteins and peptides biologically functionally equivalent to the proteins and peptides disclosed herein include amino acid sequences containing conservative amino acid changes in the fundamental amino acid sequence. In such amino acid sequences, one or more amino acids in the fundamental sequence can be substituted, for example, with another amino acid(s), the charge and polarity of which is similar to that of the native amino acid, i.e., a conservative amino acid substitution, resulting in a silent change. It should be noted that there are a number of different classification systems in the art that have been developed to describe the interchangeability of amino acids for one another within peptides, polypeptides, and proteins. The following discussion is merely illustrative of some of these systems, and the present disclosure encompasses any of the “conservative” amino acid changes that would be apparent to one of ordinary skill in the art of peptide, polypeptide, and protein chemistry from any of these different systems. Unless otherwise indicated, a particular nucleic acid sequence also implicitly encompasses conservatively modified variants thereof (e.g., degenerate codon substitutions), the complementary (or complement) sequence, and the reverse complement sequence, as well as the sequence explicitly indicated. Specifically, degenerate codon substitutions may be achieved by generating sequences in which the third position of one or more selected (or all) codons is substituted with mixed-base and/or deoxyinosine residues (see e.g., Batzer et al., Nucleic Acid Res. 19:5081 (1991); Ohtsuka et al., J. Biol. Chem. 260:2605-2608 (1985); and Rossolini et al., Mol. Cell. Probes 8:91-98 (1994)). Because of the degeneracy of nucleic acid codons, one can use various different polynucleotides to encode identical polypeptides. Table 13, infra, contains information about which nucleic acid codons encode which amino acids.

    TABLE-US-00001 TABLE 13 Amino acid Nucleic acid codons Amino Acid Nucleic Acid Codons Ala/A GCT, GCC, GCA, GCG Arg/R CGT, CGC, CGA, CGG, AGA, AGG Asn/N AAT, AAC Asp/D GAT, GAC Cys/C TGT, TGC Gln/Q CAA, CAG Glu/E GAA, GAG Gly/G GGT, GGC, GGA, GGG His/H CAT, CAC Ile/I ATT, ATC, ATA Leu/L TTA, TTG, CTT, CTC, CTA, CTG Lys/K AAA, AAG Met/M ATG Phe/F TTT, TTC Pro/P CCT, CCC, CCA, CCG Ser/S TCT, TCC, TCA, TCG, AGT, AGC Thr/T ACT, ACC, ACA, ACG Trp/W TGG Tyr/Y TAT, TAC Val/V GTT, GTC, GTA, GTG

    [0394] Any commercially or scientifically valuable plant is encompassed in accordance with some embodiments of the disclosure. Plants that are particularly useful in the methods of the disclosure, for example expression of, and/or application of sRNAs as described herein, include all plants which belong to the super family Viridiplantae, in particular monocotyledonous and dicotyledonous plants including a fodder or forage legume, ornamental plant, food crop, tree, or shrub selected from the list comprising Acacia spp., Acer spp., Actinidia spp., Aesculus spp., Agathis australis, Albizia amara, Alsophila tricolor, Andropogon spp., Arachis spp, Areca catechu, Astelia fragrans, Astragalus cicer, Baikiaea plurijuga, Betula spp., Brassica spp., Bruguiera gymnorrhiza, Burkea africana, Butea frondosa, Cadaba farinosa, Calliandra spp, Camellia sinensis, Canna indica, Capsicum spp., Cassia spp., Centroema pubescens, Chacoomeles spp., Cinnamomum cassia, Coffea arabica, Colophospermum mopane, Coronillia varia, Cotoneaster serotina, Crataegus spp., Cucumis spp., Cupressus spp., Cyathea dealbata, Cydonia oblonga, Cryptomeria japonica, Cymbopogon spp., Cynthea dealbata, Cydonia oblonga, Dalbergia monetaria, Davallia divaricata, Desmodium spp., Dicksonia squarosa, Dibeteropogon amplectens, Dioclea spp, Dolichos spp., Dorycnium rectum, Echinochloa pyramidalis, Ehraffia spp., Eleusine coracana, Eragrestis spp., Erythrina spp., Eucalyptus spp., Euclea schimperi, Eulalia vi/losa, Pagopyrum spp., Feijoa sellowlana, Fragaria spp., Flemingia spp, Freycinetia banksli, Geranium thunbergii, GinAgo biloba, Glycine javanica, Gliricidia spp, Gossypium hirsutum, Grevillea spp., Guibourtia coleosperma, Hedysarum spp., Hemaffhia altissima, Heteropogon contoffus, Hordeum vulgare, Hyparrhenia rufa, Hypericum erectum, Hypeffhelia dissolute, Indigo incamata, Iris spp., Leptarrhena pyrolifolia, Lespediza spp., Lettuca spp., Leucaena leucocephala, Loudetia simplex, Lotonus bainesli, Lotus spp., Macrotyloma axillare, Malus spp., Manihot esculenta, Medicago saliva, Metasequoia glyptostroboides, Musa sapientum, Nicotianum spp., Onobrychis spp., Ornithopus spp., Oryza spp., Peltophorum africanum, Pennisetum spp., Persea gratissima, Petunia spp., Phaseolus spp., Phoenix canariensis, Phormium cookianum, Photinia spp., Picea glauca, Pinus spp., Pisum sativam, Podocarpus totara, Pogonarthria fleckii, Pogonaffhria squamosa, Populus spp., Prosopis cineraria, Pseudotsuga menziesii, Pterolobium stellatum, Pyrus communis, Quercus spp., Rhaphiolepsis umbellata, Rhopalostylis sapida, Rhus natalensis, Ribes grossularia, Ribes spp., Robinia pseudoacacia, Rosa spp., Rubus spp., Salix spp., Schyzachyrium sanguineum, Sciadopitys vefficillata, Sequoia sempervirens, Sequoiadendron giganteum, Sorghum bicolor, Spinacia spp., Sporobolus fimbriatus, Stiburus alopecuroides, Stylosanthos humilis, Tadehagi spp, Taxodium distichum, Themeda triandra, Trifolium spp., Triticum spp., Tsuga heterophylla, Vaccinium spp., Vicia spp., Vitis vinifera, Watsonia pyramidata, Zantedeschia aethiopica, Zea mays, amaranth, artichoke, asparagus, broccoli, Brussels sprouts, cabbage, canola, carrot, cauliflower, celery, collard greens, flax, kale, lentil, oilseed rape, okra, onion, potato, rice, soybean, straw, sugar beet, sugar cane, sunflower, tomato, squash tea, maize, wheat, barley, rye, oat, peanut, pea, lentil and alfalfa, cotton, rapeseed, canola, pepper, sunflower, tobacco, eggplant, eucalyptus, a tree, an ornamental plant, a perennial grass and a forage crop. Alternatively algae and other non-Viridiplantae can be used for the methods of the present disclosure.

    [0395] According to some embodiments of the disclosure, the plant used by the method of the disclosure is a crop plant including, but not limited to, cotton, Brassica vegetables, oilseed rape, sesame, olive tree, palm oil, banana, wheat, corn or maize, barley, alfalfa, peanuts, sunflowers, rice, oats, sugarcane, soybean, turf grasses, barley, rye, sorghum, sugar cane, chicory, lettuce, tomato, zucchini, bell pepper, eggplant, cucumber, melon, watermelon, beans, hibiscus, okra, apple, rose, strawberry, chili, garlic, pea, lentil, canola, mums, Arabidopsis, broccoli, cabbage, beet, quinoa, spinach, squash, onion, leek, tobacco, potato, sugar beet, papaya, pineapple, mango, Arabidopsis thaliana, and also plants used in horticulture, floriculture or forestry, such as, but not limited to, poplar, fir, eucalyptus, pine, an ornamental plant, a perennial grass and a forage crop, coniferous plants, moss, algae, as well as other plants available on the internet at, for example, wwwdotnationmasterdotcom/encyclopedia/Plantae.

    [0396] According to a specific embodiment, the plant is selected from the group consisting of corn, rice, wheat, tomato, cotton and sorghum. In certain embodiments, the plant is a corn plant. In certain embodiments, the plant is a rice plant. In certain embodiments, the plant is a wheat plant. In certain embodiments, the plant is a cotton plant. In certain embodiments, the plant is a sorghum plant.

    [0397] The availability of sRNA fragments produced by one or more of the RNase III mutants provides a supply of a reagent or therapeutic agent and a novel therapeutic approach in which a desired knockdown effect can be achieved in a whole organism without the disadvantages of gene therapy. A gene derived from a pathogen can be targeted for inhibition. For example, the gene could cause immunosuppression of the host directly or be essential for replication of the pathogen, transmission of the pathogen or maintenance of the infection. The inhibitory RNA could be introduced in cells in vitro or ex vivo and then subsequently placed into an organism to effect therapy, or the organism could be directly treated by in vivo administration. A method of gene therapy can be envisioned. For example, cells at risk for infection by a pathogen or already infected cells, may be targeted for treatment by introduction of sRNA according to the invention. The target gene might be a pathogen or host gene responsible for entry of a pathogen into its host, drug metabolism by the pathogen or host, replication or integration of the pathogen's genome, establishment or spread of an infection in the host, or assembly of the next generation of pathogen. Methods of prophylaxis (i.e., prevention or decreased risk of infection), as well as reduction in the frequency or severity of symptoms associated with infection, can be envisioned.

    [0398] In a further embodiment, a composition including a genetically modified bacteria configured to express one or more RNase III mutants that produce sRNA may be formulated as feed and/or a water dispersible granule or powder that may further be configured to be dispersed into the environment. In yet a further embodiment, the compositions of the present invention may also comprise a wettable powder, spray, emulsion, colloid, aqueous or organic solution, dust, pellet, or colloidal concentrate. Dry forms of the compositions may be formulated to dissolve immediately upon wetting, or alternatively, dissolve in a controlled-release, sustained-release, or other time-dependent manner. Alternatively or additionally, the composition may comprise an aqueous solution. Such aqueous solutions or suspensions may be provided as a concentrated stock solution which is diluted prior to application, or alternatively, as a diluted solution ready-to-apply. Such compositions may be formulated in a variety of ways. They may be employed as wettable powders, granules or dusts, by mixing with various inert materials, such as inorganic minerals (silicone or silicon derivatives, phyllosilicates, carbonates, sulfates, phosphates, and the like) or botanical materials (powdered corncobs, rice hulls, walnut shells, and the like). The formulations or compositions containing genetically modified bacteria may include spreader-sticker adjuvants, stabilizing agents, other pesticidal additives, or surfactants. Liquid formulations may be employed as foams, suspensions, emulsifiable concentrates, or the like. The ingredients may include Theological agents, surfactants, emulsifiers, dispersants, or polymers.

    [0399] According to one embodiment, the composition is administered to the host by feeding. Feeding the host with the composition can be effected once, regularly, or semi-regularly over the span of hours, days, weeks, months or even years.

    [0400] As mentioned, the sRNA of the invention may be administered as a naked sRNA. Alternatively, the sRNA of the invention may be conjugated to a carrier known to one of skill in the art, such as a transfection agent e.g. PEI or chitosan or a protein/lipid carrier or coupled to nanoparticles. The compositions may be formulated prior to administration in an appropriate means such as lyophilized, freeze-dried, microencapsulated, desiccated, or in an aqueous carrier, medium or suitable diluent, such as saline or other buffer. Suitable agricultural carriers can be solid, semi-solid or liquid and are well known in the art. Such compositions may be considered “agriculturally-acceptable carriers”, which may covers all adjuvants, e.g., inert components, dispersants, surfactants, tackifiers, binders, etc. that are ordinarily used in pesticide formulation technology.

    [0401] The invention now being generally described will be more readily understood by reference to the following examples, which are included merely for the purposes of illustration of certain aspects of the embodiments of the present invention. The examples are not intended to limit the invention, as one of skill in the art would recognize from the above teachings and the following examples that other techniques and methods can satisfy the claims and can be employed without departing from the scope of the claimed invention. Indeed, while this invention has been particularly shown and described with references to preferred embodiments thereof, it will be understood by those skilled in the art that various changes in form and details may be made therein without departing from the scope of the invention encompassed by the appended claims.

    EXAMPLES

    Example 1: RNase III Mutants Screening Procedures

    [0402] The present inventors utilized a tetA-sacB counter selection method to screen several bacterial RNase III mutants constructed on the bacterial chromosome. Specifically, the present inventors utilizes tetA-sacB counter selection method to screen several E. coli RNase III mutants constructed on the bacterial chromosome.

    Example 2: Construction of E38A-L40F and E117K-L119F RNase III Mutants

    [0403] In one embodiment, the present inventors demonstrated the use of a wild-type Escherichia coli JM109(DE3) strain to construct E38A-L40F and E117K-L119F mutants on the bacterial chromosome. JM109 (DE3) genotype: endA1, recA1, gyrA96, thi, hsdR17 (rk−, mk+), relA1, supE44, λ-, Δ(lac-proAB), [F′, traD36, proAB, lacIqZAM15], 1DE3. TetA-sacB counter selection method was used to construct the E38A-L40F and E117K-L119F mutants as shown in FIG. 1B. In this embodiment, the plasmid pKD46 or pSIJ8, as shown in FIG. 2, was transformed into JM109 (DE3) for Red recombination.

    [0404] The present inventors initiated the following protocol: T-SACK strain was used as a template to clone tetA-sacB cassette (˜3.5 kb targeting fragment) with primers Ecoli-tet-sacB38F1 and Ecoli-tet-sacB38R1, where each primer included over 50 bp homology arms as generally shown in Table 1). The JM109 (DE3) containing pKD46 (identified at cgsc2.biology.yale.edu/Strain.php?ID=68099), or pSIJ8 (identified at addgene.org/68122/), plasmid is grown overnight at 30° C. in LB with a final concentration of 100 μg/mL ampicillin to maintain the plasmid. The overnight culture is diluted 100-fold in SOB with a final concentration of 100 μg/mL ampicillin and is grown at 30° C. to OD.sub.600˜0.3. L-arabinose is then added with a final concentration of 10 mmol/L to induce another 2 hrs to express Red enzyme, and then is used to make electro-competent cells. About 1 μg of purified tetA-sacB PCR product mixes with 100 μL competent cell for electroporation. The electroporation condition is 0.1 cm cuvette, 1.8 kV, 200Ω, and 25 μF. After electroporation, the cells are transformed into 1 mL of SOC and grown for over 4 hrs with aeration before plating on the pre-warmed (37° C.) tetracycline plate (final concentration 10 μg/mL) and then incubated for one day.

    [0405] Notably, the <tetA-sacB> designation denotes the insertion of tetA-sacB gene by recombineering within the designated position. The E38<tetA-sacB> and E117<tetA-sacB> mutants were screening with by colony PCR with specific primers JD-5 and Tet-sacB-JD-R1 as shown in FIG. 3 and Table 1. The correct E38<tetA-sacB> and E117<tetA-sacB> mutants containing the recombination plasmid are grown overnight and are used to make electro-competent cell as generally described above. About 5 μL of 10 mmol/L Ecoli-oligo-E38A or Ecoli-oligo-E117K (See Table 1) is mixed with E38<tetA-sacB> or E117<tetA-sacB> competent cells, respectively, and then electroporation is performed under the same condition as described above. After electroporation, the cells are transferred to 1 mL of SOC at 30° C. and grown for over hrs with aeration before plating on pre-warmed (37° C.) sacB agar plate and incubated for 2 days. The colony PCR with specific primer pairs Ecoli-E38A-1F and Ecoli-E38A-1R, and JD-5 and JD-3 generally identified in Table 1, are performed to screen the correct mutants E38A and E117K as shown in FIG. 4. The correct mutants were cultivated at 42° C. for overnight to eliminate pKD46 or pSIJ8 plasmid. All the mutants are confirmed by sequencing.

    [0406] As generally shown in FIG. 1B, the present inventors demonstrated that the recombination plasmids pKD46 or pSIJ8 were transformed into E. coli JM109 (DE3) strain and positive colonies were confirmed by extraction the plasmid and the restriction digestion. As further shown in FIG. 3, the tetA-sacB cassette was inserted into E. coli RNase III E38 and E117 positions, respectively. The present inventors randomly picked up 7 individual colonies for colony PCR with identification primers JD-5 and Tet-sacB-JD-R, and the expected fragment sizes are 368 bp and 605 bp, respectively. As demonstrated in FIG. 5, the correct insertions of E38<tetA-sacB> or E117<tetA-sacB> were purified at least two times and then used for E38A and E117K mutant construction. Ecoli-oligo-E38A was used to construct E38A-L40F mutant; Ecoli-oligo-E117K was used to construct E117K-L119F mutant. PCR with primer pairs of Ecoli-E38A-1F and

    [0407] Ecoli-E38A-1R (the expected PCR size 256 bp), Ecoli-E117K-1F and Ecoli-E117K-1R (the expected PCR size 323 bp) were performed to screen the correct mutants.

    Example 3: Construction of E38A and E117K RNase III Mutants

    [0408] Similar to the example of the construction of the E38A-L40F mutants, as shown in FIG. 5 and Table 1, a E38A was constructed by the present inventors with Ecoli-oligo-E38A-F2 and then screened with identification primer pair Ecoli-E38A-2F and Ecoli-E38A-1R, and JD-5 and JD-3. As also shown in FIG. 5 and Table 1, an E117K mutant was also constructed with Ecoli-oligo-E117K-F2 and then screened with identification primer pair Ecoli-E117K-2F and Ecoli-E117K-1R, and JD-5 and JD-3.

    Example 4: Construction of E65A RNase III Mutant

    [0409] Similar to example provided above related to the insertion of E38<tetA-sacB> into the bacterial chromosome, PCR was performed to clone tetA-sacB cassette with primer pair of Ecoli-tet-sacB-E65F1 and Ecoli-tet-sacB-E65R1. The tetA-sacB PCR fragments were used for homologous recombination to insert this cassette into E. coli JM109 (DE3) RNase III E65 position. The present inventors performed colony PCR was with primers JD-5 and Tet-sacB-JD-R, as identified in Table 1, to screen the correct insertion, and the expected fragment size is 449 bp (See FIG. 6). As again, shown in FIG. 6, Ecoli-oligo-E65A-F1 was used to construct the E65A mutant; primer pairs of Ecoli-E65A-1F and JD-3, JD-5 and JD-3 were used to screen the correct E65A candidate mutants.

    Example 5: Construction of Bc-E58A and Bc-E137K RNase III Mutants

    [0410] The present inventors demonstrated the construction of a Bacillus cereus 53522 E58A mutant, having three individual fragments: Pveg promoter fragment (primers Pveg-F1 and Pveg-R1 as shown in Table 2), Bc-E58A fragment I (primers Bc-E58A-F1 and Bc-E58A-R1 as shown in Table 2) and Bc-E58A (primers Bc-E58A-F2 and Bc-E58A-R2 as shown in Table 2). Fragment II was amplified by PCR using Q5® High-Fidelity DNA Polymerase. Each fragment was purified with QIAquick Gel Extraction Kit. Then the inventors assembled the three fragments with EcoRI-HF® digested pAD-WRKY-GHY7 plasmid to construct Bc-E58A mutant.

    [0411] Similar to the construction of pAD-Bc-E58A, Bc-E137K fragment I (primers Bc-E58A-F1 and Bc-E137K-R1 as shown in Table 2) and Bc-E137K fragment II (primers Bc-E137K-F1 and Bc-E58A-R2 as shown in Table 2) are amplified by PCR using Q5® High-Fidelity DNA Polymerase, and then assembled with Pveg promoter fragment and EcoRI-HF® digested pAD-43-25 plasmid using NEBuilder® HiFi DNA Assembly Cloning Kit to construct Bc-E137K mutant as demonstrated in FIG. 7). The correct mutant was then amplified by primers pAD-E58A-F1 and pAD-E58A-R1 then ligated into XhoI digested pAD-WRKY-GHY7 plasmid, and the correct mutant is labelled as pAD-Bc-E137K.

    Example 6: Construction of Additional Predicted RNase III Mutants

    [0412] Using Pveg plasmid as the template, PCR was performed to clone the Pveg promoter fragment (primers Pveg-F2 and Pveg-R2 as identified in Table 2) containing the HindIII and XhoI restriction enzyme sites on each side with Pveg-F2 and Pveg-R2 primers. The purified Pveg promoter fragment was then ligated to EcoRI-HF® digested pAD-WRKY-GHY7, and the correct vector was labelled as pAD-WRKY-GHY7-Pveg3. The predicted RNase III mutant fragments were synthesized by a third party as would be readily identified by those of ordinary skill in the art. As shown in FIG. 8, each predicted RNase III mutant fragment was ligated to the XhoI digested pAD-WRKY-GHY7-Veg3 plasmid and followed by transformation into HT115 competent cell. The positive colonies were selected on LB plates containing tetracycline (final concentration 10 μg/mL) and chloramphenicol antibiotics (final concentration 12.5 μg/mL). Primers Eco-F1 and SglyA-R1, as identified in Table 2, were used to amplify the positive mutants, with the expected PCR size of ˜1.0 kb as shown in FIG. 9. At least 2 plasmids were extracted for each predicted mutants and their sequences were independently confirmed.

    Example 7: Construction of Additional Enterobacteria RNase III Mutants

    [0413] To construct the Enterobacteria Ae003, and Ag001 RNase III mutants, the present inventors designed Ae-JD-5 and Ae-JD-3, as shown in Table 2, which have been configured to clone the complete mc gene (encoding RNase III enzyme) of these three Enterobacteria strains as shown in FIG. 10. Based on the mc gene sequences of Ae003 (SEQ ID NO. 18), Ae073 (SEQ ID NO. 19), and Ag001 (SEQ ID NO. 20), more RNase III mutants were designed by the present inventors. Primers Eco-F1 and SglyA-R1 as shown in Table 2, were used to amplify all the predicted RNase III mutants as shown in FIGS. 11 and 12, having an expected PCR size is 1.0 kb. All RNase III mutants are generally summarized in Table 3. Notably, predicted RNase III mutants were synthesize by GenScript.

    Example 8: Northern Blot Analyses of siRNA Production

    [0414] Total siRNA extracted using the MiniVana microRNA kit according to the manufacturer's instruction and then run on a 15% polyacrylamide gel electrophoresis. Table 4 lists the probes used for Northern blot analysis. The DIG Oligonucleotide 3′-End Labeling Kit, 2nd generation was used to label the oligo fragments. TMVU1-MP-F6-21, TMVU1-MP-R6-21, TMVU1-MP-F7-21, and TMVU1-MP-R7-21, again as identified in Table 4, were used as DNA markers to indicate the 21nt siRNA. Norther blot analysis is demonstrated in FIGS. 13-15, and 17.

    Example 9: qRT-PCR of dsRNA Cleavage Analysis

    [0415] As demonstrated in FIG. 16, the present inventors performed qRT-PCR of dsRNA cleavage from different E. coli RNase III mutants. Specifically, in this embodiment, the present inventors demonstrated the following: HT115-pAD-WRKY-GHY7: HT115 strain containing pAD-WRKY-GHY7 plasmid (tetracycline and chloramphenicol resistance), and it cannot digest dsRNA.

    [0416] HT115-pAD-WRKY-GHY7-E38A: HT115 strain containing pAD-WRKY-GHY7-E38A plasmid (tetracycline and chloramphenicol resistance), and E38A RNaseIII mutant can digest dsRNA into 26-29 bp small RNA; this strain can convert almost half of dsRNA into small RNAs compared to HT115-pAD-WRKY-GHY7, which cannot digest the dsRNA molecules. JM109-pAD-WRKY-GHY7: JM109 (DE3) RNaseIII E38A mutant containing pAD-WRKY GHY7 plasmid (chloramphenicol resistance), it can cleave dsRNA into 26-29 bp small RNA; this strain can convert almost 85% dsRNA into small RNAs compared to HT115-pAD-WRKY-GHY7. HT115-E38A-R107A-R108A: HT115 strain containing pAD-WRKY-GHY7-E38A-R107A-R108A plasmid (tetracycline and chloramphenicol resistance), and it can effectively cleave dsRNA into 22-23 bp small RNA; it can convert almost 95% dsRNA into small RNAs compared to HT115-pAD-WRKY-GHY7. HT115-E38A-R107E-R108E: HT115 strain containing pAD-WRKY-GHY7-E38A-R107E-R108E plasmid (tetracycline and chloramphenicol resistance), and it can cleave dsRNA into 26-29 bp small RNA and can convert almost 80% dsRNA into small RNA compared to HT115-pAD-WRKY-GHY7-E38A.

    Example 10: siRNA Sequencing Analyses and Computational Estimation of Binding Free Energies

    [0417] Six samples (each three replicates, 18 in total) were sent to GENEWIZ (South Plainfield, NJ) for sequencing. They consisted of: JM109 (wide-type E. coli), JM109-GHY7 (wide-type E. coli containing pAD-WRKY-GHY7 plasmid, targeting both TMV-GFP and movement protein gene), E38A-GHY7 (E38A mutant containing pAD-WRKY-GHY7 plasmid), E65A-GHY7 (E65A mutant containing pAD-WRKY-GHY7 plasmid), and E38A-R107A-R108A-GHY7 (E38A-R107A-R108A mutant containing pAD-WRKY-GHY7 plasmid), E38A-R107E-R108E (E38A-R107E-R108E containing pAD-WRKY-GHY7 plasmid).

    Example 11: Methods of sRNA Analysis

    [0418] Paired end Illumina sequencing data was received from GENEWIZ (South Plainfield, NJ). Paired reads were first joined using the bbmerge script from BBMap. Adapters were removed and quality trimming was then performed using Trimmomatic 0.38 with end and sliding window quality trimming. Resulting reads were filtered to include only reads of size 18 nt through 30 nt. Filtered reads were then aligned to the GHY7 gene sequence using bowtie 1.2.2 allowing for 0 mismatches on “-best” parameter settings. Alignments were converted to bam format and indexed using samtools 1.7. To identify and count RNA features, each unique RNA sequence seen was designated as a “feature” and the collection was converted to GTF format using the GenomicAlignments 1.16.0 (and rtracklayer 1.40.6 packages in R. The number of copies of each feature in each sample was then used to build a feature counts table.

    [0419] Further analyses on aligned read data were performed in R 3.5.1. Coverage plots were generated in R with the help of the Rsamtools 1.32.3 package. All other figures and plots were produced using the ggplot2 3.1.0 package. NMDS ordinations were built using the vegan package in R. Pair-wise analyses including Kruskal-Wallis (KW) tests and MANOVA type analyses including PERMANOVA and ANOSIM were performed using the vegan package in R. MANOVA type analyses were performed using 1000 permutations. Post-hoc Dunn's (DMRT) tests were performed based on significant Kruskal-Wallis tests using the dunn.test 1.5.3 package in R.

    Example 11: Methods for Estimation of Binding Free Energies Via Molecular Modeling and Simulations

    [0420] A homology model for WT E. coli RNase III was constructed using as template the crystal structure (PDB 2NUG) of WT Aquifex aeolicus RNase III in complex with dsRNA (. Modeller version 9.20 was used to generate five models of E. coli RNase III, from which the best homology model, as shown in FIG. 19, was chosen based on the lowest DOPE (Discrete Optimized Protein Energy) assessment score (Shen and Sali 2006). From this WT model, corresponding models for various mutant constructs (E38A, E65A, E38A/R107A/R108A, E38A/R107E/R108E, E38A/E65A, R107A/R108A, E65A/R107A/R108A, and E38A/E65A/R107A/R108A) were generated by introducing in silico point mutations with PyMOL version 2.3.

    [0421] All-atom MD simulations in explicit solvent were then performed for each of the E. coli RNase III dimer models in complex with dsRNA (taken from PDB 2NUG) using the Amber ff99SB-ILDN force field. For each dsRNA-bound RNase III model, TIP3P water molecules were added to fill a rhombic dodecahedral box around the protein-RNA complex, with a minimum distance of 1.0 nm from any protein or RNA atom to any edge of the simulation box. Monovalent sodium and chloride ions were added to each system in order to neutralize the total charge and to reach a physiological ionic strength of 150 mM. Molecular dynamics (MD) simulations were then performed for each of these systems using the Amber MD engine version 16 that has been GPU-optimized for simulating explicit solvent systems. A cut-value of 8 Å was used for calculating short-range pairwise Coulomb and Lennard Jones interaction energies. Long-range electrostatics were calculated with the PME (Particle Mesh Ewald) method (. Bonds containing hydrogen atoms were constrained using the SHAKE algorithm. A hydrogen mass repartitioning approach allowed the used of a 4-fs time step. Temperature was maintained at 310 K via Langevin dynamics with a collision frequency of 1.0 ps.sup.−1, while isotropic pressure coupling was set at 1 bar using a Monte Carlo barostat with a relaxation time of 4.0 ps. Each system was energy minimized using steepest descent for 500 steps followed by conjugant gradient for 500 steps. This was followed by equilibration under NVT ensemble conditions at 310 K for 1 ns, and then by equilibration under NPT ensemble conditions at 1 bar and 310 K for 1 ns. All protein and RNA heavy atoms had position restraints of 5000 kcal/mol.Math.Å.sup.2 up to this point. These position restraints were removed for the production runs, which were performed for 250 ns per simulation.

    [0422] To estimate absolute and relative (to WT) binding free energies for each E. coli RNase III model to dsRNA, the MM-GBSA (Molecular Mechanics—Generalized Born Surface Area) computational technique was employed via the MMPBSA.py tool. Changes in the conformational entropy were not considered here due to the high computational cost yet low predictive accuracy. The nonpolar portion of the desolvation energy was calculated using the LCPO (Linear Combinations of Pairwise Overlaps) method, with the surface tension and offset parameters set at the Amber-default values of 0.0072 and 0, respectively. The polar portion of the desolvation energy was computed and compared between five Generalized Born (GB) models and atomic radii parameters: i) GB1 with ‘mbondi’ radii, ii) GB2 with ‘mbondi2’ radii, iii) GB5 with ‘mbondi2’ radii, iv) GB7 with ‘bondi’ radii, and v) GB8 with ‘mbondi3’ radii. Prior to processing, all water molecules and monovalent ions were stripped from each frame from all simulation trajectories. The ionic strength was set at 150 mM in the GB calculations for each frame.

    TABLE-US-00002 TABLE 1 Primers used for RNase III mutant construction. Primers Sequences (5.fwdarw.3) Purpose Ecoli-tet- GAACTGTTGCAGCAGGCATTAACTCATCGTA PCR amplification of sacB38F1 GTGCCAGCAGTAAACATAACGAGTCCTAAT tetA-sacB cassette TTTTGTTGACACTCTATC (SEQ ID NO. 62) Ecoli-tet- CGCATTGGCGATAACGTAGCTCAGAATAGAG sacB38R1 TCGCCTAAAAATTCTAAACGATCAAAGGGA AAACTGTCCATATGC (SEQ ID NO. 63) Ecoli-oligo- G*T*A*G*CTCAGAATAGAGTCGCCTAAAAAT Construction of E38A- E38A TCGAAGCGGGCATTGTGTTTACTGCTGGCAC L40F mutant TACGATGAGTTAATGC (SEQ ID NO. 64) Ecoli-E38A-1F AGTAAACACAATGCCCGCTTC (256 bp) Identification of E38A- (SEQ ID NO. 65) L40F mutant Ecoli-E38A-1R ATGCTTCGACGGTGTCGG (SEQ ID NO. 66) Ecoli-tet- CTTAAAAGCGGTGGATTTCGTCGTGAGTCAA PCR amplification of sacB117F1 TTCTCGCCGACACCGTCGAATCCTAATTTTT tetA-sacB cassette GTTGACACTCTATC (SEQ ID NO. 67) Ecoli-tet- TAATTTCTCGACGGTTTGAATATCACTGTCGA sacB117R1 GGAATACGCCACCAATTAATGCATCAAAGG GAAAACTGTCCATATGC (SEQ ID NO. 68) Ecoli-oligo- T*T*G*A*ATATCACTGTCGAGGAATACGCCA Construction of E117K- E117K CCGATGAAAGCCTTCACGGTGTCGGCGAGAA L119F mutant TTGACTCACGACGAAA (SEQ ID NO. 69) Ecoli-E117K-1F GACACCGTGAAGGCTTTCATC (323 bp) Identification of E117K- (SEQ ID NO. 70) L119F mutant Ecoli-E117K-1R TTCAACGCCTGTTCGGC (SEQ ID NO. 71) Ecoli-oligo-E38A- G*T*A*G*CTCAGAATAGAGTCGCCTAAAAAT Construction of E38A F2 TCCAAGCGGGCATTGTGTTTACTGCTGGCAC mutant TACGATGAGTTAATGC (SEQ ID NO. 72) Ecoli-E38A-2F AGTAAACACAATGCCCGCTTG (SEQ ID NO. Identification of E38A 73) mutant Ecoli-oligo-E117K- T*T*G*A*ATATCACTGTCGAGGAATACGCCA Construction of E117K F2 CCGATCAAAGCCTTCACGGTGTCGGCGAGAA mutant TTGACTCACGACGAAA (SEQ ID NO. 74) Ecoli-E117K-2F GACACCGTGAAGGCTTTGATC (SEQ ID NO. Identification of E117K 75) mutant Ecoli-tet-sacB- AGCTACGTTATCGCCAATGCGCTTTATCACC PCR amplification of E65F1 GTTTCCCTCGTGTGGATGAATCCTAATTTTT tetA-sacB cassette GTTGACACTCTATC (SEQ ID NO. 76) Ecoli-tet-sacB- CGCCAGCGTATTGCCACGGACCAGCGTGGCG E65R1 CGCATCCGGCTCATATCGCCATCAAAGGGA AAACTGTCCATATGC (SEQ ID NO. 77) Ecoli-oligo-E65A- C*A*G*C*GTGGCGCGCATCCGGCTCATATCG Construction of E65A F1 CCGGCGTCGACGCGGGGGAAACGGTGATAA mutant AGCGCATTGGCGATAAC (SEQ ID NO. 78) Ecoli-E65A-1F TTTCCCCCGCGTCGACGC (SEQ ID NO. 79) Identification of E65A mutant JD-5 ACCGGTAAACTGAAACTGCA (SEQ ID NO. 80) Identification of tetA- Tet-sacB-JD-R1 TGGCAAGACTGGCATGATAAG (SEQ ID NO. sacB cassette insertion 81) into the bacterial chromosome JD-3 TGGAGATTTTCTGCCCCAG (SEQ ID NO. 82) Used for identification of mutants Note: *denoting the phosphorothioated primers.

    TABLE-US-00003 TABLE 1b Single-stranded RNAs used for Northern blot of FIG. 14 TMVU1-MP-F6-RNA21 CAGUUCAAGGUCGUUCCCAAU (SEQ ID NO. 83) TMVU1-MP-F7-RNA23 UGAAGAUGUCAGCGGGUUUCU GU (SEQ ID NO. 84) TMVU1-MP-R6-RNA25 CCAGACGUUUUUCAUCGCGUC CUGG (SEQ ID NO. 85) TMVU1-MP-R7-RNA27 ACGACUUCUUCUGUAAGUUCC AUGGGC (SEQ ID NO. 86) TMVU1-MP-F6-RNA29 CAGUUCAAGGUCGUUCCCAAU UAUGCUAU (SEQ ID NO. 87)

    TABLE-US-00004 TABLE 2 Primers used for RNase III mutants constructed in a plasmid. Primers Sequences (5.fwdarw.3) Purpose Pveg-F1 ATCACGAGGCCCTTTCGTCTTCAAGGGAGTTCTGA PCR amplification of Pveg GAATTGGTATGC (SEQ ID NO. 88) promoter Pveg-R1 ACACCTCCTTTACTACATTTATTGTACAACACGAG C (SEQ ID NO. 89) Pveg-F2 ATCACGAGGCCCTTTCGTCTTCAAGAAGCTTGGAG PCR amplification of Pveg TTCTGAGAATTGGTATGC (SEQ ID NO. 90) promoter Pveg-R2 ACGCGATCCCCGGGTACCGAGCTCGCTCGAGACAC CTCCTTTACTACATTTATTGTACAACACGAGC (SEQ ID NO. 91) Bc-E58A-F1 ACAATAAATGTAGTAAAGGAGGTGTATGCCGTACC PCR amplification of Bc- GAAAATATAGAG (SEQ ID NO. 92) E58A fragment I Bc-E58A-R1 GAGGCGGGCGTTGTCTTCATGCGGTTTTTTTCG (SEQ ID NO. 93) Bc-E58A-F2 ACCGCATGAAGACAACGCCCGCCTCGAATTTCTTG PCR amplification of Bc- GAGATGCAGTATTG (SEQ ID NO. 94) E58A fragment II Bc-E58A-R2 ACGCGATCCCCGGGTACCGAGCTCGTTATAGTTGT TCTTTTAATTTTTTCAATG (SEQ ID NO. 95) Bc-E137K-R1 GATGAAGGCCTTGAAGACATCCGCTAATAAAGCTG PCR amplification of Bc- G (SEQ ID NO. 96) E137K fragment I Bc-E137K-F1 AGCGGATGTCTTCAAGGCCTTCATCGGTGCCCTTT PCR amplification of Bc- ATCTTGATCAAG (SEQ ID NO. 97) E137K fragment II pAD-E58A-F1 CAATAAATGTAGTAAAGGAGGTGTCATGCCGTACC PCR amplification of Bc- GAAAATATAGAG (SEQ ID NO. 98) E58A or Bc-137K mutants pAD-E58A-R1 GCGAGCTCGGTACCCGGGGATCGCGTTATAGTTGT TCTTTTAATTTTTTCAATG (SEQ ID NO. 99) Eco-F1 ACGAGGCCCTTTCGTCTTCAA (SEQ ID NO. 100) pAD43-25 vector primer SglyA-R1 CATGTTCGCTTGTGCACCA (SEQ ID NO. 101) pAD43-25 vector primer Ae-JD-5 AACTAACGACATCCCCTGTCGT (SEQ ID NO. 102) PCR amplification of Ae-JD-3 CGCAGCTTGTTCAGCACCAT (SEQ ID NO. 103) bacterial rnc gene

    TABLE-US-00005 TABLE 3 Summary of RNase III mutants Label Mutations Function References M- E38A-L40F Mutations in the bacterial This JM109- chromosome, produced discrete 26- study GHY7 29 bp siRNAs, higher Mg.sup.2+ M- Ec-E38A Mutations in the bacterial This (Xiao et al., 2009) JM109- chromosome, produced discrete 26- study GHY7 29 bp siRNAs M- HT115-E38A- Mutations constructed in a plasmid, This JM109- K12opt produced discrete 26-29 bp siRNAs study GHY7 M- HT115-E38A- Mutations constructed in a plasmid, This JM109- R107A-R108A produced 22-23 bp siRNA study GHY7 M- HT115-Ag001- Mutations constructed in a plasmid, This JM109- E38A produced discrete 26-29 bp siRNA study GHY7 M- HT115-Ag001- Mutations constructed in a plasmid, This JM109- E38A-R107A- produced 22-23 bp siRNA study GHY7 R108A M- HT115-Ag1- Mutations constructed in a plasmid, This JM109- E38A-R86C- produced 22-23 bp siRNA, the study GHY7 R107A-R108A cleavage efficiency is decreased compared to Ag1-E38A-R107A- R108A M- HT115-Ae003- Mutations constructed in a plasmid, This JM109- E38A produced discrete 26-29 bp siRNA study GHY7 M- HT115-Ae003- Mutations constructed in a plasmid, This JM109- E38A-R107A- produced 22-23 bp siRNA study GHY7 R108A M- E65A Mutations in the bacterial This JM109- chromosome, 26-29 bp siRNAs study GHY7 M- E117K-L119F Mutations in the bacterial This JM109- chromosome, produced dsRNA study GHY7 binding without cleavage M- E117K (rnc70) Mutations in the bacterial (Cao et al., 2013, JM109- chromosome, not functional in Dasgupta et al., 1998, GHY7 dsRNA cleavage but remained the Inada et al., 1989, Li & dsRNA binding activity Nicholson, 1996) M- HT115-E117Q Mutations constructed in a plasmid, (Sun & Nicholson, JM109- not functional in dsRNA cleavage but 2001) GHY7 remained the dsRNA binding activity M- HT115-E117D Mutations constructed in a plasmid, (Sun & Nicholson, JM109- not functional in dsRNA cleavage and 2001) GHY7 binding M- HT115-Q153P Mutations constructed in a plasmid, (Inada & Nakamura, JM109- not functional in dsRNA cleavage but 1995) GHY7 remained the dsRNA binding activity M- HT115-D155E Mutations constructed in a plasmid, (Inada & Nakamura, JM109- not functional in dsRNA cleavage and 1995) GHY7 binding M- HT115-E38A- Mutations constructed in a plasmid This JM109- ΔS33-R107A- study GHY7 R108A M- HT115-E38A- Mutations constructed in a plasmid This JM109- S33A-ΔS34- study GHY7 R107A-R108A M- HT115-E38A- Mutations constructed in a plasmid This JM109- ΔA32-ΔS33- study GHY7 ΔS34 M- HT115-E38A- Mutations constructed in a plasmid, This JM109- ΔA32-ΔS33- possible 22-23 bp siRNA, the band is study GHY7 ΔS34-K35V very weak, under the threshold sensitivity of Northern blot analysis M- HT115-E38A- Mutations constructed in a plasmid, This JM109- ΔS33-ΔS34- possible 22-23 bp siRNA, the band is study GHY7 ΔK35 very weak, under the threshold sensitivity of Northern blot analysis M- HT115-E30A Mutations constructed in a plasmid, This JM109- study GHY7 M- HT115-E30A- Mutations constructed in a plasmid, This JM109- K12opt study GHY7

    TABLE-US-00006 TABLE 4 Sequences of probes and primers for Northern blot analysis and qRT-PCR. Name Sequence (5′.fwdarw.3′) TMVMP-probe1s TCTCGGATCTTACTACACAGCAGCTGCAAAGAA AAGATTTCAGTT (SEQ ID NO. 104) TMVMP-probe2as TCCTGGGTGGTTATAGCATAATTGGGAACGACC TTGAACTGAAAT SEQ ID NO. 105) TMVMP-probe3s CACCCAGGACGCGATGAAAAACGTCTGGCAAGT TTTAGTTAATAT SEQ ID NO. 106) TMVMP-probe4as AGCGGACAGAAACCCGCTGACATCTTCACATTT CTAATATTAACT SEQ ID NO. 107) TMVMP-probe5s CTGTCCGCTTTCTCTGGAGTTTGTGTCGGTGTG TATTGTTTATAG SEQ ID NO. 108) TMVMP-probe6as CCCTCCGTCTCTCACGTTTGTAATCTTCTCTCT CAAACCTAATTT SEQ ID NO. 109) TMVMP-probe8as CTTTGCAAGCCTGATCGACATAGGGACATCTTC CATGAACTCATC SEQ ID NO. 110) TMVMP-probe9s GTTTCGATCTCGAACCGGAAAAAAGAGTGATGT CCGCAAAGGGAA SEQ ID NO. 111) TMVU1-MP-F6-21 CAGTTCAAGGTCGTTCCCAAT SEQ ID  NO. 112) TMVU1-MP-R6-21 GTTTTTCATCGCGTCCTGGGT SEQ ID  NO. 113) TMVU1-MP-F7-21 AAGATGTCAGCGGGTTTCTGT SEQ ID  NO. 114) TMVU1-MP-R7-21 CTTCTTCTGTAAGTTCCATGG SEQ ID  NO. 115) TMVU1-MP-F4 CCAGGACGCGATGAAAAACG SEQ ID  NO. 118) TMVU1-MP-R4 GGACAGAAACCCGCTGACAT SEQ ID  NO. 119) Ec-16SrRNA-F1 GAATGCCACGGTGAATACGTT SEQ ID  NO. 120) Ec-16SrRNA-R1 ACCCACTCCCATGGTGTGA SEQ ID  NO. 121)

    TABLE-US-00007 TABLE 5 sRNA processed an aligned read information Sample Total_Counts Aligned_Counts Prop_aligned Treatment 1 Treatment2 Replicate E38A-GHY7-1 19875890 1536686 0.077314072476755 dsRNA E38A 1 E38A-GHY7-2 20887014 1892870 0.090624251029851 dsRNA E38A 2 E38A-GHY7-3 22395853 2077999 0.092784990149739 dsRNA E38A 3 E38A-R107E-R108E-GHY7-1 17856798 696574 0.039008897339826 dsRNA R-mut-E 1 E38A-R107E-R108E-GHY7-2 13744950 481533 0.035033448648413 dsRNA R-mut-E 2 E38A-R107E-R108E-GHY7-3 17651690 944198 0.053490515639013 dsRNA R-mut-E 3 E38A-R107A-R108A-GHY7-1 19176252 1940405 0.10118791722178 dsRNA R-mut-A 1 E38A-R107A-R108A-GHY7-2 20952849 1611653 0.076918084027618 dsRNA R-mut-A 2 E38A-R107A-R108A-GHY7-3 19414442 1000029 0.051509541196188 dsRNA R-mut-A 3 E65A-GHY7-1 23274731 2929987 0.125887040327126 dsRNA E65A 1 E65A-GHY7-2 25562644 3354559 0.131228952685802 dsRNA E65A 2 E65A-GHY7-3 20078044 2373409 0.118209174160591 dsRNA E65A 3 JM109-1 16103261 12680 0.000787418150895 no Wild-type 1 dsRNA JM109-2 16273933 15556 0.000955884481029 no Wild-type 2 dsRNA JM109-3 17383893 15654 0.00090048874553 no Wild-type 3 dsRNA JM109-GHY7-1 13439306 413319 0.030754489852378 dsRNA Wild-type 1 JM109-GHY7-2 14691724 435247 0.029625318308457 dsRNA Wild-type 2 JM109-GHY7-3 18607641 476936 0.025631190971494 dsRNA Wild-type 3

    TABLE-US-00008 TABLE 6 Manova-type Test Results Test Type Test Statistic p-value PERMANOVA F = 191.19 <0.01 ANOSIM R = ~1     <0.01

    TABLE-US-00009 TABLE 7 Summary of select RNase III mutations showing increase catalytic activity and preferred sRNA production results. SEQ ID NO. Mutant Rnase III Results Size Preference 3, 4 E38A E. coli Catalytic improvement 26, 29 nt 5, 6 E65A E. coli Catalytic improvement 26, 29 nt 17 E38A-E65A E. coli Catalytic improvement 26, 29 nt 7, 8 E38A-R107A-R108A E. coli Catalytic improvement and 22, 23 nt cutting enhancement 11, 12 E38A-R107A-R108A Enterobacteriaceae Ag001 Able to cut dsRNA 22, 23 nt  9, 10 E38A Enterobacteriaceae Ag001 Able to cut dsRNA 26, 29 nt 15, 16 E38A-R107A-R108A Enterobacter Ae003 Able to cut dsRNA 22, 23 nt 13, 14 E38A Enterobacter Ae003 Able to cut dsRNA 26, 29 nt 37, 38 Q153P E. coli Able to cut dsRNA non-WT  39, 40 D155E E. coli Able to cut dsRNA non-WT  55, 56 E58A B. cereus Able to cut dsRNA non-WT* 57, 58 E59A B. subtilus Able to cut dsRNA non-WT* 27, 28 E117K E. coli Binds but does not cut dsRNA NA *nonWT cutting expected based on homology to E38 in RNase III in E. Coli

    TABLE-US-00010 TABLE 8 Target pathogens in poultry populations Poultry Viral diseases Fungal diseases Parasitic diseases Chickens Avian influenza (has Aspergillosis (genus: Coccidiosis (genus: Turkeys multiple strains or types, and Aspergillus) Eimeria) Ducks is divided into three types: A, B, and C; H5N1 (genus: Influenzavirus A) can cause a 90-100% mortality) Newcastle Disease (genus: Candidiasis (genus: Ascaridia galli (genus: Avulavirus) Candida) Ascaridia) Poxvirus diseases (mainly Blackhead (genus: genera: Parapoxvirus, Histomonas) orthopoxvirus, yatapoxvirus, molluscipoxvirus) Infectious bronchitis virus Mites (genus: (IBV) (genus: Dermanyssus) Gammacoronavirus) Laryngotracheitis (genus: Lice (genus: Menophon) Iltovirus) Marek's Disease (genus: Mardivirus) Eastern Equine Encephalitis (genus: Alphavirus) Hemorrhagic enteritis (genus: Siadenovirus) Viral arthritis (genus: Reovirus)

    TABLE-US-00011 TABLE 9 Target pathogens in bee populations Bees (Apis Mellifera) Viral diseases Fungal diseases Parasitic diseases Dicistroviruses: Nosema apis - causing Varroa mite (Varroa nosemosis, the most destructor). common adult honey bees disease. Israeli acute paralysis Ascosphaera apis Honey bee tracheal virus (CCD (Colony (causing Chalkbrood mites (Acarapis woodi) Collapse Syndrom)) disease) Kashmir bee virus Aspegillus spp (causing Small hive beetles (Aethina (CCD) Stonebrood disease) tumida) - colonies damage in non-apis bees (bumble bees and stingless bees) Acute bee paralysis Tropilaelaps mites virus (CCD) (Tropilaelaps mercedesae) Black queen cell virus Wax moth (Pyralidae: Galleria (affect pupae but not Mellonela and Achroia grisella) adults) Aphid lethal paralysis virus (possibly CCD) Big sioux river virus (possibly CCD) Iflaviruses: Deformed wing virus Kakugo virus Varroa destructor virus-1 Sacbrood virus Thai/Chinese sacbrood virus Slow bee paralysis virus Baculovirus: Apis iridescent virus (CCD) Unclassified viruses: Cloudy wing virus Bee virus-X Bee virus-Y Lake Sinai virus-1 Lake Sinai virus-2

    TABLE-US-00012 TABLE 10 Target pathogens in mammal populations Mammal Diseases Bluetongue Virus (BTV): Affects sheep, goats, deer and cattle Bovine Viral Diarrhoea (BVD): Cattle and other ruminants Calf Pneumonia: Caused by bovine Respiratory Syncytial Vims (bRSV), Parainfluenza III Vims (PI3) Infectious Bovine Rhinotracheitis (IBR): Caused by Bovine Herpesvirus-1 (BHV-1) Trypanosomosis (Sleeping disease): Affects both human and animals. Transmitted through tse-tse fly by flagellated protozoan parasites. The most economically important livestock disease of Africa Foot-and-mouth disease Virus (FMDV): Highly contagious viral disease that affects cattle and swine. It also affects sheep, goats, deer, and other cloven-hooved ruminants Rift Valley Fever Virus: viral disease of cattle and sheep. It is spread through infected mosquitoes. It can spread to humans either as airborne and/or by consuming raw milk, handling undercooked meat. Rotaviral Diarrhoea: Caused by bovine Rotavirus Parasitic gastro-enteritis (PGE or Gut worms): Affect cattle and is spread through parasites (abomasal worms) Anaplasmosis: Vector-borne, infectious blood disease in cattle caused by the rickettsial parasites Anaplasma marginale and Anaplasma centrale. It is also known as yellow-bag or yellow-fever Bovine Anaemia: Benign theileriosis is a tick-borne disease caused by intracellular blood parasites belonging to the Theileria orientalis group (BATOG) Bovine Babesiosis (BB) (Redwater, Tick Fever): Tick-borne disease of cattle. Caused by single-cell parasites mainly babesia bovis and babesia bigemma, with Rhipicephalus ticks being the major vector Rabies (Rabies Virus): Affects cattles and other ruminants. It is transmitted through the biting of infected animals such as foxes, dogs, skunks and raccoons, but mostly by bat carrying rabies Neosporosis: Caused by the protozoan Neospora caninum. Affects cattle and sheep. Hosts are canids such as dogs and foxes Schmallenberg Virus (SBV): New emerging disease. Affects cattle, bison, sheep and goats. Transmitted through midges and vertically from dam to offspring Epizootic Hemorrhagic Disease Virus (EHDV): Most important infectious disease of white-tailed deer in US. It affects also antelope, mule and other deer species. Cattles are affected uncommonly. It is spread by biting flies (midges, gnats) Lice: Affects cattle and other ruminants. Two types of lice, biting and sucking lice Mange: Cattles and other ruminants are infected by mites Pseudocowpox: Caused by a parapox virus. Most common infectious cause of teat disease in cattle Ringworm: Skin disease affecting cattles and other ruminants. It is caused by Trichophyton verrucosum fungi Ulcerative mammillitis: Affects cattle. Caused by a herpes virus (BHV-2) Orf disease: Affects primarily sheep and goats. Caused by a parapox virus Toxoplasmosis: Affects sheep. Caused by the Toxoplasma gondii parasite. Coccidiosis: Affects cattle, sheep, chicken, dogs. Caused by Coccidian parasites Myiasis: Parasitic infestation of a live mammal by fly larvae (maggots). Affects a wide range of mammals such as humans, sheep, horse, rabbit Louping ill: Acute, tick-transmitted viral disease that affects goats, horses, dogs, pigs, sheep, cattle. Caused by louping ill virus Echinococcosis: Affects sheep goats, cattle, swine, kangaroos, canids such as dogs and foxes, cats and wild felids. Parasitic disease caused by infection with tiny tapeworms of the genus Echinocococcus Fasciolosis: Parasitic worm infection caused by the common liver fluke Fasciola hepatica as well as by Fasciola gigantica. Affects human, sheep and cattle. It is a plant-borne zoonosis Coenurosis: Parasitic infection that develops in the intermediate hosts of some tapeworm species (Taenia multiceps, T. serialis, T. brauni, or T. glomerate) and are caused by the coenurus, the larval stage of these worms. Affects sheep and other ungulates but also humans Caprine arthritis and encephalitis Virus (CAEV): Affects goats Chagas (TRYPANOSOMA CRUZI): Affects human, horses, cattle and goats. Caused by the parasites trypanosomes Myxomatosis: Caused by Myxoma virus, transmitted through insect (mosquito, fly, fur mite) bites. Affects rabbits Ear mites (canker): Affect rabbits. Caused by the mite Psoroptes cuniculi. Encephalitozoon Cuniculi: Affect rabbits. Caused by single-cell protozoan parasite Fleas: Ectoparasites Rabbitpox: Affects rabbits. Caused by rabbitpox virus (RPXV) Viral Haemorrhagic Disease: Also known as rabbit Haemorrhagic Disease (RHD). Caused by a calicivirus. Affects rabbits Swine Influenza: Affects pigs. Cause by Swine Influenza virus (SIV) Japanese B Encephalitis Virus (JE): Affects pigs, transmitted through mosquitoes Trichinosis: Parasitic disease caused by roundworms of Trichinella. Affects pigs Encephalomyocarditis Virus (EMCV): Affects pigs, transmitted through rats Swine pox: Caused by Swine pox virus, affects pigs Porcine Parvovirus Infection (PPV): Most common and important cause of infectious infertility in pigs Porcine Respiratory Corona Virus Infection (PRCV) Porcine Cytomegalovirus Infection (PCMV) Transmissible Gastro Enteritis (TGE): Caused by a coronavirus. Affects pigs Enteroviruses, SMEDI: gut-borne viruses. Affects pigs Aujeszky's disease (AD): Caused by a herpes virus, affects pigs Nipah virus disease: Causes death both in humans and pigs. New disease, first identified in Malaysia in 1998. Caused by a previously unknown paramyxovirus Swine Fevers; African, Classical, Hog Cholera Viruses: Affects pigs Teschen Disease: Caused by a porcine enterovirus serotype 1

    [0423] In one preferred embodiment, the present invention may be applied to one or more of the following non-limiting group of plant viruses, including pathogen gene targets, generally referred to as gene targets, or essential genes, which would be recognized and available to those of ordinary skill in the art without undue experimentation:

    TABLE-US-00013 TABLE 11 Target plant viral pathogens Plant Pathogens Virus diseases hosts Pathogenic genes References Tobacco mosaic virus Tobacco, tomato, and Replicase gene, (Scholthof, 2004) (TMV) other solanaceous movement protein, plants. It can infect coat protein well over 350 different species of plants. The typical symptoms are necrosis, mosaic, mottling, stunting, leaf curling, and yellowing of plant tissues, etc. Tomato spotted wilt Over 1,000 species in glycoproteins (GPs), (Adkins, 2000) virus over 85 families, NSm protein, NSs (TSWV) including many protein, virus RNA vegetables, peanut, genomic segment L, and tobacco, are M, and S. susceptible to TSWV. The Solanaceae and Compositae families contain the largest numbers of susceptible plant species. TSWV also replicates in its insect vector, thrips (Thysanoptera: Thripidae) Tomato yellow leaf Plants are stunted or V1, V2, C1, C2, C3, (Czosnek, 2007) curl virus dwarfed, can infect and C4. V1 protein (TYLCV) about 50 different plant species Cucumber mosaic Over 1,200 species in 1a, 2a and 2b protein, (Palukaitis & García- virus (CMV) over 100 families of 3a and coat protein Arenal, 2003) monocots and dicots, including many vegetables, ornamentals and woody and semi- woody plants Potato virus Y (PVY) PVY mostly infects P1, HC-Pro, P3, 6k1, (Jakab et al., 1997) plants in the family CI, 6k2, NIa, Nib, Solanaceae. The and CP Solanaceous plants include economically important ones like potato (Solanum tuberosum), as well as tomato, tomatillo, green pepper, chili pepper, eggplant, petunia and many weeds, such as the nightshades. Easily spread by aphids Cauliflower mosaic CaMV infects mostly Movement protein, (Hoh et al., 2010) virus (CaMV) plants of the two aphid Brassicaceae family transmission factors (such as cauliflower (P2 and P3), the and turnip) but some precursor of the CaMV strains (D4 capsid proteins (P4), and W260) are also and polyprotein able to infect precursor of Solanaceae species of proteinase, P5, and the genera Datura and P6 protein. Nicotiana. African cassava Mosaic, leaf AV1, AV2, AC1, (Bock & Harrison, mosaic virus distortion and AC2, AC3, AC4, 1985, Fauquet & (ACMV) stunting BC1, BV1 Fargette, 1990) Plum pox virus (PPV) Prunus species is P1, HC-Pro, P3, 6k1, (Cambra et al., 2006, widespread in most CI, 6k2, NIa, Nib, Ilardi & Tavazza, stone fruit-producing and CP 2015) countries. Symptoms include chlorotic and necrotic ring patterns or blotches Brome mosaic virus BMV is cosmopolitan 1a, 2a, movement (Miller et al., 1985, (BMV) and found virtually protein, coat protein Ahlquist & Janda, wherever wheat is 1984) grown. Potato virus X (PVX) PVX is found mainly Replicase, TGB1, (Kaniewski et al., in potatoes and is TGB2, TGB3, and 1990, Kutnjak et al., only transmitted coat protein 2014) mechanically, most infections are transmitted by farm machinery, can also be transmitted by vectors such as grasshoppers or biting insects

    [0424] Additional plant pathogens may include: Citrus tristeza virus, Barley yellow dwarf virus, Potato leafroll virus and Tomato and bushy stunt virus.

    [0425] In one preferred embodiment, the present invention may be applied to one or more of the following non-limiting group of plant fungal pathogens, including pathogen gene targets, generally referred to as gene targets, or essential genes, which would be recognized and available to those of ordinary skill in the art without undue experimentation:

    TABLE-US-00014 TABLE 12 Target fungal pathogens Plant Pathogens hosts Pathogenic genes References Maguaporthe Rice (Oryza sativa). MoABC1, MoMAC1 and MoPMK1, (Zhu et al., oryzae pathogenicity-related genes, 2017, Dong effectors Iug6, Iug9 and Iug18, et al., 2015) secreted proteins: MoMpg1, MoEmp1, MoMhp1, MoMsp1, MC69, and Slp1, etc. Botrytis cinerea It can infect over 200 pathogenicity-related genes Bcpg1 (Williamson plant species, causing and BMP1 et al., 2007, grey mould, evident on Have et al., the surface as grey 1998, Zheng fluffy mycelium. et al., 2000) Worldwide, it causes annual losses of $10 billion to $100 billion. Puccinia spp. Wheat and barley, pathogenicity-related genes (Stakman & common barberry (and MAPK, cyclophilin, and Levine, 1944, some additional calcineurin regulatory subunit, and Chen, 2005, Berberis, Mahoberberis, secreted proteins etc. Rampitsch et and Mahonia spp.) al., 2006, Panwar et al., 2013, Cantu et al., 2013) Fusarium Wheat (Triticum MAP1, and MAP kinase gpmk1 (Goswami & graminearum aestivum), Durum etc. Kistler, 2004, Wheat (Triticum Urban et al., durum), Barley 2003, (Hordeum vulgare) and Jenczmionka Oat (Avena sativa). F. et al., 2003) graminearum parasitizes roots, stems, leaves, and reproductive tissues of many species of cereals and grasses. Fusarium It can infect many plants MAP kinase, pg1, pathogenicity- (Di Pietro et oxysporum including potato, related genes, secreted proteins, al., 2001, sugarcane, garden bean, etc. Michielse & cowpea, Prickly pear, Rep, 2009, cultivated zinnia, pansy, Di Pietro & Assam rattlebox, Baby's Roncero, breath, and Musa sp. 1998) Blumeria Causing powdery effector gene Avra10, (Nowara et graminis mildew on grasses, pathogenicity-related genes, al., 2010, including cereals. secreted proteins, etc. Bindschedler et al., 2016) Mycosphaerella causing septoria leaf pathogenicity-related genes, (Goodwin et graminicola blotch, in most years is MgSlt2, ABC Transporter Genes al., 2011, the second most MgAtr1 and MgAtr2, secreted Brading et important disease of proteins, etc. al., 2002, wheat in the United Mehrabi et States al., 2006, Zwiers & De Waard, 2000) Colletotrichum black spot disease in the CMK1, and clk1, pathogenesis- (Cannon et spp. common bean plant related protein 10, secreted al., 2012, proteins, etc. Takano et al., 2000, Dufresne et al., 1998, Lo et al., 1999) Ustilago maydis causing smut on maize pathogenicity-related genes, Kpp2, (Kämper et and teosinte ukc1, secreted proteins, etc. al., 2006, Müller et al., 1999, Dürrenberger & Kronstad, 1999) Melampsora flax rust pathogenicity-related genes, (Flor, 1956, lini secreted proteins, etc. Lawrence et al., 1981, Nemri et al., 2014)

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    SEQUENCES

    [0484] As noted above, the instant application contains a full Sequence Listing which has been submitted electronically in XML format and is hereby incorporated by reference in its entirety. The following sequences are further provided herewith and are hereby incorporated into the specification in their entirety:

    TABLE-US-00015 DNA E.coli-JM109(DE3)-wild-type-681 bp E. coli SEQ ID NO. 1 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACATAACGAGCGTTTAGAATTTTTAGGCGACTCTAT TCTGAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGG ATGCGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCT TACGTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTCGA AGCATTAATTGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTAT CAAACTCGTTTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATT TGCAGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGA ATTTACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAG GCTGAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid E.coli-JM109(DE3)-wild-type-226 aa E. coli SEQ ID NO. 2 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNERLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA M-JM109-GHY7-Ec-E38A E. coli SEQ ID NO. 3 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACACAATGCCCGCTTGGAATTTTTAGGCGACTCTAT TCTGAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGG ATGCGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCT TACGTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTCGA AGCATTAATTGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTAT CAAACTCGTTTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATT TGCAGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGA ATTTACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAG GCTGAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid M-JM109-GHY7-Ec-E38A-aa E. coli SEQ ID NO. 4 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA M-JM109-GHY7-E65A E. coli SEQ ID NO. 5 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACATAACGAGCGTTTAGAATTTTTAGGCGACTCTAT TCTGAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCCCGCGTCGACGCCGGCGATATGAGCCGG ATGCGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCT TACGTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTCGA AGCATTAATTGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTAT CAAACTCGTTTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATT TGCAGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGA ATTTACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAG GCTGAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid M-JM109-GHY7-E65A-aa E. coli SEQ ID NO. 6 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNERLEFLGDSILSYVIANALYHRFPRVDAGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA HT115-E38A-R107A-R108A E. coli SEQ ID NO. 7 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACACAATGCCCGCTTGGAATTTTTAGGCGACTCTAT TCTGAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGG ATGCGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCT TACGTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTGCCGCCGAGTCAATTCTCGCCGACACCGTCGA AGCATTAATTGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTAT CAAACTCGTTTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATT TGCAGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGA ATTTACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAG GCTGAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid HT115-E38A-R107A-R108A-aa E. coli SEQ ID NO. 8 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFAAESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA HT115-Ag001-E38A Enterobacteriaceae Ag001 SEQ ID NO. 9 ATGAATCCCATCGTAATAAATAGGCTGCAGCGTAAGCTGGGCTACACTTTTCAACATCAGGATCTGTTGC AACAGGCATTAACCCATCGGAGTGCCAGCAGCAAGCATAATGCCCGCTTGGAGTTTTTGGGTGACTCCAT TCTCAGTTATGTCATCGCGAATGCGCTGTATCATCGTTTTCCTCGCGTAGATGAAGGCGACATGAGCCGC ATGCGTGCGACGCTGGTGCGCGGCAATACGCTGGCGGAAATCGCCCGCGAGTTCGAACTGGGTGAGTGTC TGCGTCTTGGGCCGGGTGAACTGAAAAGTGGCGGTTTCCGTCGCGAGTCGATTCTTGCTGATACCGTGGA AGCGTTGATCGGTGGCGTCTTCCTCGACAGCGACATTCAGAACGTTGAGCGTTTGATTCTCTCGTGGTAT CAGACCCGTCTCGACGAAATCAGTCCAGGCGACAAGCAAAAAGATCCGAAAACGCGTCTGCAGGAGTACC TGCAGGGTCGCCATCTGCCGCTGCCGTCGTATCTGGTGGTGCAGGTGCGTGGTGAAGCGCACGATCAAGA ATTTACCATTCACTGTCAGGTGAGTGGCCTGCCTGAGCCTGTCGTAGGGACGGGCTCAAGCCGCCGTAAA GCGGAACAGGCTGCGGCTGAGCAGGCACTGAAAAAGCTGGAGCTGGAATGA Amino Acid HT115-Ag001-E38A-aa Enterobacteriaceae Ag001 SEQ ID NO. 10 MNPIVINRLQRKLGYTFQHQDLLQQALTHRSASSKHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAEIAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQNVERLILSWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPSYLVVQVRGEAHDQEFTIHCQVSGLPEPVVGTGSSRRK AEQAAAEQALKKLELE DNA HT115-Ag001-E38A-R107A-R108A Enterobacteriaceae Ag001 SEQ ID NO. 11 ATGAATCCCATCGTAATAAATAGGCTGCAGCGTAAGCTGGGCTACACTTTTCAACATCAGGATCTGTTGC AACAGGCATTAACCCATCGGAGTGCCAGCAGCAAGCATAATGCCCGCTTGGAGTTTTTGGGTGACTCCAT TCTCAGTTATGTCATCGCGAATGCGCTGTATCATCGTTTTCCTCGCGTAGATGAAGGCGACATGAGCCGC ATGCGTGCGACGCTGGTGCGCGGCAATACGCTGGCGGAAATCGCCCGCGAGTTCGAACTGGGTGAGTGTC TGCGTCTTGGGCCGGGTGAACTGAAAAGTGGCGGTTTCGCCGCCGAGTCGATTCTTGCTGATACCGTGGA AGCGTTGATCGGTGGCGTCTTCCTCGACAGCGACATTCAGAACGTTGAGCGTTTGATTCTCTCGTGGTAT CAGACCCGTCTCGACGAAATCAGTCCAGGCGACAAGCAAAAAGATCCGAAAACGCGTCTGCAGGAGTACC TGCAGGGTCGCCATCTGCCGCTGCCGTCGTATCTGGTGGTGCAGGTGCGTGGTGAAGCGCACGATCAAGA ATTTACCATTCACTGTCAGGTGAGTGGCCTGCCTGAGCCTGTCGTAGGGACGGGCTCAAGCCGCCGTAAA GCGGAACAGGCTGCGGCTGAGCAGGCACTGAAAAAGCTGGAGCTGGAATGA Amino Acid HT115-Ag001-E38A-R107A-R108A-aa Enterobacteriaceae Ag001 SEQ ID NO. 12 MNPIVINRLQRKLGYTFQHQDLLQQALTHRSASSKHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAEIAREFELGECLRLGPGELKSGGFAAESILADTVEALIGGVFLDSDIQNVERLILSWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPSYLVVQVRGEAHDQEFTIHCQVSGLPEPVVGTGSSRRK AEQAAAEQALKKLELE DNA HT115-Ae003-E38A Enterobacter Ae003 SEQ ID NO. 13 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTCATCATCAGGAGTTGTTGC AACAGGCATTAACCCACCGCAGTGCCAGCAGCAAGCACAACGCCCGCCTGGAGTTTTTAGGCGACTCTAT TTTAAGTTTCGTGATTGCGAATGCGCTTTATCATCGTTTCCCGCGCGTGGATGAAGGTGATATGAGCCGC ATGCGTGCCACGCTGGTTCGGGGTAACACCCTTGCGGAAATCGCGCGCGAATTTGAACTGGGCGAATGTC TGCGTCTTGGGCCGGGTGAACTGAAAAGCGGCGGCTTCCGTCGTGAATCTATTCTTGCCGATACGGTCGA AGCATTAATTGGTGGTGTGTTCCTGGACAGCGATATCCAGACCGTCGAAAAGCTGATCCTGAACTGGTAT CAGACCCGTCTGGACGAAATCAGCCCGGGCGATAAACAAAAAGATCCCAAAACGCGTCTGCAGGAATATT TGCAGGGCCGTCATCTGCCGCTGCCATCTTATCTGGTGGTGCAGGTTCGTGGCGAAGCGCACGATCAGGA ATTTACCATCCATTGCCAGGTCAGTGGCCTGAGTGAACCGGTGGTGGGCACAGGTTCAAGCCGTCGTAAG GCTGAACAGGCTGCCGCCGAACAGGCGTTAAAAATGCTGGAGCTGGAATGA Amino Acid HT115-Ae003-E38A-aa Enterobacter Ae003 SEQ ID NO. 14 MNPIVINRLQRKLGYTFHHQELLQQALTHRSASSKHNARLEFLGDSILSFVIANALYHRFPRVDEGDMSR MRATLVRGNTLAEIAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPSYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKMLELE DNA HT115-Ae003-E38A-R107A-R108A Enterobacter Ae003 SEQ ID NO. 15 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTCATCATCAGGAGTTGTTGC AACAGGCATTAACCCACCGCAGTGCCAGCAGCAAGCACAACGCCCGCCTGGAGTTTTTAGGCGACTCTAT TTTAAGTTTCGTGATTGCGAATGCGCTTTATCATCGTTTCCCGCGCGTGGATGAAGGTGATATGAGCCGC ATGCGTGCCACGCTGGTTCGGGGTAACACCCTTGCGGAAATCGCGCGCGAATTTGAACTGGGCGAATGTC TGCGTCTTGGGCCGGGTGAACTGAAAAGCGGCGGCTTCGCCGCCGAATCTATTCTTGCCGATACGGTCGA AGCATTAATTGGTGGTGTGTTCCTGGACAGCGATATCCAGACCGTCGAAAAGCTGATCCTGAACTGGTAT CAGACCCGTCTGGACGAAATCAGCCCGGGCGATAAACAAAAAGATCCCAAAACGCGTCTGCAGGAATATT TGCAGGGCCGTCATCTGCCGCTGCCATCTTATCTGGTGGTGCAGGTTCGTGGCGAAGCGCACGATCAGGA ATTTACCATCCATTGCCAGGTCAGTGGCCTGAGTGAACCGGTGGTGGGCACAGGTTCAAGCCGTCGTAAG GCTGAACAGGCTGCCGCCGAACAGGCGTTAAAAATGCTGGAGCTGGAATGA Amino Acid HT115-Ae003-E38A-R107A-R108A-aa Enterobacter Ae003 SEQ ID NO. 16 MNPIVINRLQRKLGYTFHHQELLQQALTHRSASSKHNARLEFLGDSILSFVIANALYHRFPRVDEGDMSR MRATLVRGNTLAEIAREFELGECLRLGPGELKSGGFAAESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPSYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKMLELE Amino Acid RNase III E38A-E65A mutant E. coli SEQ ID NO. 17 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNARLEFLGDSILSYVIANALYHRFPRVDAGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA Ae003-rnc Enterobacteria SEQ ID NO. 18 AACTAACGACATCCCCTGTCGTTGTGTATAGAATATTCCCCCGAAGTTTAAGGTTGGCCCTGCAAGGGTG CCACGGCACACGAAACCGCGTTGGTTTTCTCAGGTCGGTTTCGTGTGCTGCATTTTTGACGCATTCATTT ATTGGTATCGCATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTCATCATCA GGAGTTGTTGCAACAGGCATTAACCCACCGCAGTGCCAGCAGCAAACATAATGAGCGTCTCGAGTTTTTA GGCGACTCTATTTTAAGTTTCGTGATTGCGAATGCGCTTTATCATCGTTTCCCGCGCGTGGATGAAGGTG ATATGAGCCGCATGCGTGCCACGCTGGTTCGGGGTAACACCCTTGCGGAAATCGCGCGCGAATTTGAACT GGGCGAATGTCTGCGTCTTGGGCCGGGTGAACTGAAAAGCGGCGGCTTCCGTCGTGAATCTATTCTTGCC GATACGGTCGAAGCATTAATTGGTGGTGTGTTCCTGGACAGCGATATCCAGACCGTCGAAAAGCTGATCC TGAACTGGTATCAGACCCGTCTGGACGAAATCAGCCCGGGCGATAAACAAAAAGATCCCAAAACGCGTCT GCAGGAATATTTGCAGGGCCGTCATCTGCCGCTGCCATCTTATCTGGTGGTGCAGGTTCGTGGCGAAGCG CACGATCAGGAATTTACCATCCATTGCCAGGTCAGTGGCCTGAGTGAACCGGTGGTGGGCACAGGTTCAA GCCGTCGTAAGGCTGAACAGGCTGCCGCCGAACAGGCGTTAAAAATGCTGGAGCTGGAATGAGCGAAGAA AAGACCTATTGCGGATTTATTGCCATCGTCGGACGTCCGAACGTCGGCAAATCCACCCTGTTGAATAATC TGCTTGGGCAGAAGATTTCTATCACCTCGCGTAAGGCTCAGACCACGCGTCACCGCATCGTCGGTATCCA TACTGAAGGCGCGTATCAGGCGATCTACGTCGATACCCCGGGCCTGCACATGGAAGAGAAGCGTGCCATC AACCGTCTGATGAACAAGGCGGCGAGCAGCTCGATTGGCGACGTGGAGCTGGTGATTTTCGTTGTGGAAG GCACCCGCTGGACGCCTGACGACGAGATGGTGCTGAACAAGCTGCG DNA Ae073-rnc Enterobacteria SEQ ID NO. 19 AACTAACGACATCCCCTGTCGTTGTGTATAGAATATTCCCCCGAAGTTTAAGGTTGGCCCTGCAAGGGTG CCACGGCACACGAAACCGCGTTGGTTTTCTCAGGTCGGTTTCGTGTGCTGCATTTTTGACGCATTCATTT ATTGGTATCGCATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTCATCATCA GGAGTTGTTGCAACAGGCATTAACCCACCGCAGTGCCAGCAGCAAACATAATGAGCGTCTCGAGTTTTTA GGCGACTCTATTTTAAGTTTCGTGATTGCGAATGCGCTTTATCATCGTTTCCCGCGCGTGGATGAAGGTG ATATGAGCCGCATGCGTGCCACGCTGGTTCGGGGTAATACCCTTGCGGAAATCGCGCGCGAATTTGAGCT GGGCGAATGTCTGCGTCTTGGGCCGGGTGAACTGAAAAGCGGCGGCTTCCGTCGTGAATCTATTCTTGCC GATACGGTCGAAGCATTAATTGGTGGTGTGTTCCTGGACAGCGATATCCAGACCGTCGAAAAGCTGATCC TGAACTGGTATCAGACCCGTCTGGACGAAATCAGCCCGGGCGATAAACAAAAAGATCCCAAAACGCGTCT GCAGGAATATTTGCAGGGCCGTCATCTGCCGCTGCCATCTTATCTGGTGGTGCAGGTTCGTGGCGAAGCG CACGATCAGGAATTTACCATCCATTGCCAGGTCAGTGGCCTGAGTGAACCGGTGGTGGGCACAGGTTCAA GCCGTCGTAAGGCTGAACAGGCTGCCGCCGAACAGGCGTTAAAAATGCTGGAGCTGGAATGAGCGAAGAA AAGACCTATTGCGGATTTATTGCCATCGTCGGACGTCCGAACGTCGGCAAATCCACCCTGTTGAATAATC TGCTTGGGCAGAAGATTTCTATCACCTCGCGTAAGGCGCAGACCACGCGTCACCGCATCGTCGGTATCCA TACTGAAGGCGCGTATCAGGCGATCTACGTCGATACACCGGGCCTGCACATGGAAGAGAAGCGTGCCATC AACCGTCTGATGAACAAGGCGGCGAGCAGCTCAATTGGCGACGTGGAGCTGGTGATTTTCGTTGTGGAAG GCACCCGCTGGACGCCGGACGACGAGATGGTGCTGAACAAGCTGCG DNA Ag001-rnc Enterobacteria SEQ ID NO. 20 AACTAACGACATCCCCTGTCGTTGTGTATAGAATATTCCCGCCTTTAAAGATTGGCTCCCGAAAGGGAGC CACGGCACACGAAACAGCGTTGGTTTCCTTTTTTCAGGTCTGTTCCGTGTGCTGAATAGTTGACGCATTC ATTAATTTTGGTATCGCATGAATCCCATCGTAATAAATAGGCTGCAGCGTAAGCTGGGCTACACTTTTCA ACATCAGGATCTGTTGCAACAGGCATTAACCCATCGGAGTGCCAGCAGCAAACACAACGAGCGTCTTGAG TTTTTGGGTGACTCCATTCTCAGTTATGTCATCGCGAATGCGCTGTATCATCGTTTTCCTCGCGTAGATG AAGGCGACATGAGCCGCATGCGTGCGACGCTGGTGCGCGGCAATACGCTGGCGGAAATCGCCCGCGAGTT CGAACTGGGTGAGTGTCTGCGTCTTGGGCCGGGTGAACTGAAAAGTGGCGGTTTCCGTCGCGAGTCGATT CTTGCTGATACCGTGGAAGCGTTGATCGGTGGCGTCTTCCTCGACAGCGACATTCAGAACGTTGAGCGTT TGATTCTCTCGTGGTATCAGACCCGTCTCGACGAAATCAGTCCAGGCGACAAGCAAAAAGATCCGAAAAC GCGTCTGCAGGAGTACCTGCAGGGTCGCCATCTGCCGCTGCCGTCGTATCTGGTGGTGCAGGTGCGTGGT GAAGCGCACGATCAAGAATTTACCATTCACTGTCAGGTGAGTGGCCTGCCTGAGCCTGTCGTAGGGACGG GCTCAAGCCGCCGTAAAGCGGAACAGGCTGCGGCTGAGCAGGCACTGAAAAAGCTGGAGCTGGAATGAGC GAAGAAAAAACGTATTGCGGCTTCGCGGCCATTGTTGGTCGCCCGAACGTCGGCAAATCCACGCTGCTGA ATCAGCTGCTTGGGCAAAAAGTTTCCATTACCTCGCGTAAGGCGCAAACCACGCGCCACCGCATCATGGG CATCCATACCGAAGGGCCATATCAGGCGATTTACGTCGATACCCCGGGGCTGCACATGGAAGAAAAACGC GCCATTAACCGCCTGATGAACCGCGCGGCAAGCAGCTCCATCGGTGACGTTGAGCTGGTTATCTTCGTGG TTGAAGGCACCCGCTGGACGCCGGATGATGAAATGGTGCTGAACAAGCTGCG Amino Acid Ag001-rnc Enterobacteria SEQ ID NO. 21 MNPIVINRLQRKLGYTFQHQDLLQQALTHRSASSKHNERLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAEIAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQNVERLILSWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPSYLVVQVRGEAHDQEFTIHCQVSGLPEPVVGTGSSRRK AEQAAAEQALKKLELE Amino Acid Ae003-rnc Enterobacteria SEQ ID NO. 22 MNPIVINRLQRKLGYTFHHQELLQQALTHRSASSKHNERLEFLGDSILSFVIANALYHRFPRVDEGDMSR MRATLVRGNTLAEIAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPSYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKMLELE DNA Verrucomicrobia-rnc-wide-type Verrucomicrobia SEQ ID NO. 23 ATGAATCCGCTCGAAGACCGCATCGGTTACAAGTTCCGCAACGCGCTGTTGCTGGAAGAAGCGCTCACGC ATCCCAGTGTGAGGCACGAGCGCCTGGAGTTTTTGGGCGATGCGGTCCTGCAGCTCGTGATGACGGAACA CCTGTTCGGGCATTTTAAGAAAGAAGCCGAAGGGACGCTGACGAAACTGCGCTCGCGGCTTGTTTCGCGG GAGGCCCTCGCCGTTCATGCGGCGACGCTCGAACTGGGACGCTATCTGGCCGTCGGCCGCGGTGAGGACG CGAGCGGCGGTCGCGAACGCAATTCGACGCTCGCCGACGCTTTCGAGGCGCTCGTCGGAGCGATCTATCT CGATAGCGATCTGGCCACGGTGCGTCGCTTTATCCTGGATCAGGCAGCGGGCGATCTGGCGCAACTCGTC GACGAACCGACCGATATCAACCCGAAGGGTCACCTGCAGGAATTGCTCCAGGCGATTTCGCCCCGCAGCC CGGTTTACGAAGTGATTTCGCAGACCGGGCCGGAGCACGAAAAGACGTTTGTGATTCGCGCGGTTTGGGA GGGCATCACGCTCGGGGAGGGAACCGGGCGAAGCAAGAAACAGGCGGAAACGGCCGCCGCCGAGGAGGCG ATGCGGCAAAAGCGGTGGGAAACGGAAAAGACGTCGACCGCACCTTCTCGGTAG Amino Acid Verrucomicrobia-rnc-wide-type-aa Verrucomicrobia SEQ ID NO. 24 MNPLEDRIGYKFRNALLLEEALTHPSVRHERLEFLGDAVLQLVMTEHLFGHFKKEAEGTLTKLRSRLVSR EALAVHAATLELGRYLAVGRGEDASGGRERNSTLADAFEALVGAIYLDSDLATVRRFILDQAAGDLAQLV DEPTDINPKGHLQELLQAISPRSPVYEVISQTGPEHEKTFVIRAVWEGITLGEGTGRSKKQAETAAAEEA MRQKRWETEKTSTAPSR DNA M-JM109-GHY7-E117K-L119F E. coli SEQ ID NO. 25 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACATAACGAGCGTTTAGAATTTTTAGGCGACTCTAT TCTGAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGG ATGCGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCT TACGTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTGAA GGCTTTCATCGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTAT CAAACTCGTTTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATT TGCAGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGA ATTTACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAG GCTGAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid M-JM109-GHY7-E117K-L119F-aa E. coli SEQ ID NO. 26 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNERLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVKAFIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA M-JM109-GHY7-Ec-E117K E. coli SEQ ID NO. 27 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACATAACGAGCGTTTAGAATTTTTAGGCGACTCTAT TCTGAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGG ATGCGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCT TACGTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTGAA GGCTTTGATCGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTAT CAAACTCGTTTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATT TGCAGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGA ATTTACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAG GCTGAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid M-JM109-GHY7-Ec-E117K-aa E. coli SEQ ID NO. 28 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNERLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVKALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA HT115-E38A-K12opt E. coli SEQ ID NO. 29 ATGAATCCCATCGTGATCAACCGTTTGCAGCGTAAATTGGGTTACACTTTTAATCACCAAGAATTGCTGC AGCAGGCATTGACCCACCGCTCCGCTTCGTCTAAACACAACGCCCGTCTGGAATTTTTAGGAGATTCGAT CCTGTCTTACGTGATCGCCAATGCACTGTATCACCGCTTTCCCCGCGTGGATGAAGGAGATATGAGCCGT ATGCGTGCGACACTTGTGCGCGGAAATACCCTGGCAGAACTGGCGCGCGAGTTCGAACTGGGAGAGTGCT TACGCCTTGGTCCCGGTGAGCTGAAGTCCGGGGGCTTTCGTCGTGAGTCTATCCTTGCTGATACGGTTGA AGCTTTAATCGGGGGTGTATTTTTAGACTCAGACATCCAAACAGTGGAAAAGCTTATCTTGAACTGGTAC CAAACCCGTTTAGATGAGATCAGCCCGGGGGACAAACAAAAGGACCCAAAGACACGTTTGCAGGAGTACC TTCAAGGGCGTCACCTGCCCTTGCCAACATACTTAGTAGTCCAGGTACGTGGAGAAGCACACGATCAGGA GTTCACCATTCACTGTCAAGTTAGTGGGTTATCCGAACCTGTAGTGGGGACGGGCTCCTCACGTCGCAAA GCGGAACAAGCTGCGGCTGAACAGGCATTGAAAAAATTGGAGCTTGAGTAA Amino Acid HT115-E38A-K12opt-aa E. coli SEQ ID NO. 30 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA Ag001-E38A-R86C-R107A-R108A Enterobacteriaceae SEQ ID NO. 31 ATGAATCCCATCGTAATAAATAGGCTGCAGCGTAAGCTGGGCTACACTTTTCAACATCAGGATCTGTTGC AACAGGCATTAACCCATCGGAGTGCCAGCAGCAAGCATAATGCCCGCTTGGAGTTTTTGGGTGACTCCAT TCTCAGTTATGTCATCGCGAATGCGCTGTATCATCGTTTTCCTCGCGTAGATGAAGGCGACATGAGCCGC ATGCGTGCGACGCTGGTGCGCGGCAATACGCTGGCGGAAATCGCCTGCGAGTTCGAACTGGGTGAGTGTC TGCGTCTTGGGCCGGGTGAACTGAAAAGTGGCGGTTTCGCCGCCGAGTCGATTCTTGCTGATACCGTGGA AGCGTTGATCGGTGGCGTCTTCCTCGACAGCGACATTCAGAACGTTGAGCGTTTGATTCTCTCGTGGTAT CAGACCCGTCTCGACGAAATCAGTCCAGGCGACAAGCAAAAAGATCCGAAAACGCGTCTGCAGGAGTACC TGCAGGGTCGCCATCTGCCGCTGCCGTCGTATCTGGTGGTGCAGGTGCGTGGTGAAGCGCACGATCAAGA ATTTACCATTCACTGTCAGGTGAGTGGCCTGCCTGAGCCTGTCGTAGGGACGGGCTCAAGCCGCCGTAAA GCGGAACAGGCTGCGGCTGAGCAGGCACTGAAAAAGCTGGAGCTGGAATGA Amino Acid Ag001-E38A-R86C-R107A-R108A-aa Enterobacteriaceae SEQ ID NO. 32 MNPIVINRLQRKLGYTFQHQDLLQQALTHRSASSKHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAEIACEFELGECLRLGPGELKSGGFAAESILADTVEALIGGVFLDSDIQNVERLILSWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPSYLVVQVRGEAHDQEFTIHCQVSGLPEPVVGTGSSRRK AEQAAAEQALKKLELE DNA HT115-E117Q E. coli SEQ ID NO. 33 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACATAACGAGCGTTTAGAATTTTTAGGCGACTCTAT TCTGAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGG ATGCGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCT TACGTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACGGTGCA GGCTTTGATCGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTAT CAAACTCGTTTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATT TGCAGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGA ATTTACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAG GCTGAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid HT115-E117Q-aa E. coli SEQ ID NO. 34 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNERLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVQALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA HT115-E117D E. coli SEQ ID NO. 35 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACATAACGAGCGTTTAGAATTTTTAGGCGACTCTAT TCTGAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGG ATGCGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCT TACGTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACGGTGGA CGCTTTGATCGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTAT CAAACTCGTTTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATT TGCAGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGA ATTTACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAG GCTGAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid HT115-E117D-aa E. coli SEQ ID NO. 36 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNERLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVDALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA HT115-Q153P E. coli SEQ ID NO. 37 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACATAACGAGCGTTTAGAATTTTTAGGCGACTCTAT TCTGAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGG ATGCGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCT TACGTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTCGA AGCATTAATTGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTAT CAAACTCGTTTGGACGAAATTAGCCCAGGCGACAAGCCCAAGGACCCGAAAACGCGCTTGCAAGAATATT TGCAGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGA ATTTACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAG GCTGAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid HT115-Q153P-aa E. coli SEQ ID NO. 38 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNERLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKPKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA HT115-D155E E. coli SEQ ID NO. 39 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACATAACGAGCGTTTAGAATTTTTAGGCGACTCTAT TCTGAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGG ATGCGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCT TACGTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTCGA AGCATTAATTGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTAT CAAACTCGTTTGGACGAAATTAGCCCAGGCGACAAGCAGAAGGAGCCCAAAACGCGCTTGCAAGAATATT TGCAGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGA ATTTACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAG GCTGAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid HT115-D155E-aa E. coli SEQ ID NO. 40 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASSKHNERLEFLGDSILSYVIANALYHRFPRVDEGDMSR MRATLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWY QTRLDEISPGDKQKEPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRK AEQAAAEQALKKLELE DNA HT115-E38A-ΔS33-R107A-R108A E. coli SEQ ID NO. 41 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCAGTAAACACAATGCCCGCTTGGAATTTTTAGGCGACTCTATTCT GAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGGATG CGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCTTAC GTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTGCCGCCGAGTCAATTCTCGCCGACACCGTCGAAGC ATTAATTGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTATCAA ACTCGTTTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATTTGC AGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGAATT TACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAGGCT GAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid HT115-E38A-ΔS33-R107A-R108A-aa E. coli SEQ ID NO. 42 MNPIVINRLQRKLGYTFNHQELLQQALTHRSASKHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSRM RATLVRGNTLAELAREFELGECLRLGPGELKSGGFAAESILADTVEALIGGVFLDSDIQTVEKLILNWYQ TRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRKA EQAAAEQALKKLELE DNA HT115-E38A-S33A-ΔS34-R107A-R108A E. coli SEQ ID NO. 43 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCGCCAAACACAATGCCCGCTTGGAATTTTTAGGCGACTCTATTCT GAGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGGATG CGCGCCACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCTTAC GTTTAGGGCCAGGTGAACTTAAAAGCGGTGGATTTGCCGCCGAGTCAATTCTCGCCGACACCGTCGAAGC ATTAATTGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTATCAA ACTCGTTTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATTTGC AGGGTCGCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGAATT TACTATCCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAGGCT GAGCAGGCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid HT115-E38A-S33A-ΔS34-R107A-R108A-aa E. coli SEQ ID NO. 44 MNPIVINRLQRKLGYTFNHQELLQQALTHRSAAKHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSRM RATLVRGNTLAELAREFELGECLRLGPGELKSGGFAAESILADTVEALIGGVFLDSDIQTVEKLILNWYQ TRLDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRKA EQAAAEQALKKLELE DNA HT115-E38A-ΔA32-ΔS33-ΔS34 E. coli SEQ ID NO. 45 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTAAACACAATGCCCGCTTGGAATTTTTAGGCGACTCTATTCTGAGCTA CGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGGATGCGCGCC ACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCTTACGTTTAG GGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTCGAAGCATTAAT TGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTATCAAACTCGT TTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATTTGCAGGGTC GCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGAATTTACTAT CCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAGGCTGAGCAG GCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid HT115-E38A-ΔA32-ΔS33-ΔS34-aa E. coli SEQ ID NO. 46 MNPIVINRLQRKLGYTFNHQELLQQALTHRSKHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSRMRA TLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWYQTR LDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRKAEQ AAAEQALKKLELE DNA HT115-E38A-ΔA32-ΔS33-ΔS34-K35V E. coli SEQ ID NO. 47 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGTACACAATGCCCGCTTGGAATTTTTAGGCGACTCTATTCTGAGCTA CGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGGATGCGCGCC ACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCTTACGTTTAG GGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTCGAAGCATTAAT TGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTATCAAACTCGT TTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATTTGCAGGGTC GCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGAATTTACTAT CCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAGGCTGAGCAG GCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid HT115-E38A-ΔA32-ΔS33-ΔS34-K35V-aa E. coli SEQ ID NO. 48 MNPIVINRLQRKLGYTFNHQELLQQALTHRSVHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSRMRA TLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWYQTR LDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRKAEQ AAAEQALKKLELE DNA HT115-E38A-ΔS33-ΔS34-ΔK35 E. coli SEQ ID NO. 49 ATGAACCCCATCGTAATTAATCGGCTTCAACGGAAGCTGGGCTACACTTTTAATCATCAGGAACTGTTGC AGCAGGCATTAACTCATCGTAGTGCCCACAATGCCCGCTTGGAATTTTTAGGCGACTCTATTCTGAGCTA CGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAAGGCGATATGAGCCGGATGCGCGCC ACGCTGGTCCGTGGCAATACGCTGGCGGAACTGGCGCGCGAATTTGAGTTAGGCGAGTGCTTACGTTTAG GGCCAGGTGAACTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTCGAAGCATTAAT TGGTGGCGTATTCCTCGACAGTGATATTCAAACCGTCGAGAAATTAATCCTCAACTGGTATCAAACTCGT TTGGACGAAATTAGCCCAGGCGATAAACAAAAAGATCCGAAAACGCGCTTGCAAGAATATTTGCAGGGTC GCCATCTGCCGCTGCCGACTTATCTGGTAGTCCAGGTACGTGGCGAAGCGCACGATCAGGAATTTACTAT CCACTGCCAGGTCAGCGGCCTGAGTGAACCGGTGGTTGGCACAGGTTCAAGCCGTCGTAAGGCTGAGCAG GCTGCCGCCGAACAGGCGTTGAAAAAACTGGAGCTGGAATGA Amino Acid HT115-E38A-ΔS33-ΔS34-ΔK35-aa E. coli SEQ ID NO. 50 MNPIVINRLQRKLGYTFNHQELLQQALTHRSAHNARLEFLGDSILSYVIANALYHRFPRVDEGDMSRMRA TLVRGNTLAELAREFELGECLRLGPGELKSGGFRRESILADTVEALIGGVFLDSDIQTVEKLILNWYQTR LDEISPGDKQKDPKTRLQEYLQGRHLPLPTYLVVQVRGEAHDQEFTIHCQVSGLSEPVVGTGSSRRKAEQ AAAEQALKKLELE DNA HT115-E30A Verrucomicrobia SEQ ID NO. 51 ATGAATCCGCTCGAAGACCGCATCGGTTACAAGTTCCGCAACGCGCTGTTGCTGGAAGAAGCGCTCACGC ATCCCAGTGTGAGGCACGCGCGCCTGGAGTTTTTGGGCGATGCGGTCCTGCAGCTCGTGATGACGGAACA CCTGTTCGGGCATTTTAAGAAAGAAGCCGAAGGGACGCTGACGAAACTGCGCTCGCGGCTTGTTTCGCGG GAGGCCCTCGCCGTTCATGCGGCGACGCTCGAACTGGGACGCTATCTGGCCGTCGGCCGCGGTGAGGACG CGAGCGGCGGTCGCGAACGCAATTCGACGCTCGCCGACGCTTTCGAGGCGCTCGTCGGAGCGATCTATCT CGATAGCGATCTGGCCACGGTGCGTCGCTTTATCCTGGATCAGGCAGCGGGCGATCTGGCGCAACTCGTC GACGAACCGACCGATATCAACCCGAAGGGTCACCTGCAGGAATTGCTCCAGGCGATTTCGCCCCGCAGCC CGGTTTACGAAGTGATTTCGCAGACCGGGCCGGAGCACGAAAAGACGTTTGTGATTCGCGCGGTTTGGGA GGGCATCACGCTCGGGGAGGGAACCGGGCGAAGCAAGAAACAGGCGGAAACGGCCGCCGCCGAGGAGGCG ATGCGGCAAAAGCGGTGGGAAACGGAAAAGACGTCGACCGCACCTTCTCGGTAG Amino Acid HT115-E30A-aa Verrucomicrobia SEQ ID NO. 52 MNPLEDRIGYKFRNALLLEEALTHPSVRHARLEFLGDAVLQLVMTEHLFGHFKKEAEGTLTKLRSRLVSR EALAVHAATLELGRYLAVGRGEDASGGRERNSTLADAFEALVGAIYLDSDLATVRRFILDQAAGDLAQLV DEPTDINPKGHLQELLQAISPRSPVYEVISQTGPEHEKTFVIRAVWEGITLGEGTGRSKKQAETAAAEEA MRQKRWETEKTSTAPSR DNA HT115-E30A-K12opt Verrucomicrobia SEQ ID NO. 53 ATGAATCCTTTAGAAGACCGTATTGGGTATAAGTTTCGTAATGCTTTACTGCTGGAAGAAGCTTTGACCC ACCCATCTGTGCGCCACGCTCGTTTGGAGTTCTTGGGAGACGCGGTGTTACAATTAGTAATGACAGAACA CCTGTTCGGGCACTTTAAGAAAGAAGCTGAAGGGACTTTAACGAAACTTCGTAGCCGTTTGGTTTCCCGC GAGGCTCTGGCTGTCCACGCTGCCACTTTGGAACTTGGACGTTATTTGGCTGTGGGCCGTGGCGAGGACG CATCCGGCGGACGTGAGCGTAACTCAACGTTAGCGGACGCCTTCGAGGCTCTGGTGGGCGCGATTTATCT TGATTCAGACCTGGCAACCGTTCGTCGCTTTATTCTTGATCAGGCTGCAGGGGATTTGGCACAGTTGGTA GATGAACCGACCGATATTAACCCTAAAGGTCATTTACAGGAACTTTTGCAGGCTATCTCCCCTCGTTCCC CAGTATATGAAGTTATCTCTCAAACTGGTCCAGAACACGAAAAGACATTCGTAATCCGCGCAGTATGGGA GGGTATCACTTTAGGGGAGGGAACGGGACGCAGTAAAAAACAAGCTGAGACGGCAGCTGCTGAGGAAGCT ATGCGCCAAAAGCGTTGGGAGACGGAGAAAACTTCCACGGCCCCTTCCCGTTAA Amino Acid HT115-E30A-K12opt-aa Verrucomicrobia SEQ ID NO. 54 MNPLEDRIGYKFRNALLLEEALTHPSVRHARLEFLGDAVLQLVMTEHLFGHFKKEAEGTLTKLRSRLVSR EALAVHAATLELGRYLAVGRGEDASGGRERNSTLADAFEALVGAIYLDSDLATVRRFILDQAAGDLAQLV DEPTDINPKGHLQELLQAISPRSPVYEVISQTGPEHEKTFVIRAVWEGITLGEGTGRSKKQAETAAAEEA MRQKRWETEKTSTAPSR DNA B.cereus-E58A B. cereus SEQ ID NO. 55 ATGCCGTACCGAAAATATAGAGAAAAAAAATACGAAACAAAATATCGTGAAGCATTTAAAGTGTTTCAAG AAAAGATAGGTATTACGTTTACAGATGAAAAATTATTGATTCAAGCATTTACGCATTCATCGTATGTGAA TGAGCATCGAAAAAAACCGCATGAAGACAACGCCCGCCTCGAATTTCTTGGAGATGCAGTATTGGAACTT ACTGTATCGCAGTATCTGTTTCAAAAATATCCGACAATGAGCGAAGGAGAGTTAACAAAACTACGTGCAG CTATTGTATGTGAGCCATCTCTTGTTCGTTTTGCGAACGAATTGTCATTTGGTAGCCTTGTTTTATTAGG AAAAGGTGAAGAAATGACAGGTGGACGTGAACGACCAGCTTTATTAGCGGATGTCTTTGAAGCGTTTATT GGTGCCCTTTATCTTGATCAAGGGTTAGAAACAGTTTGGGAATTCTTAAAAGAAATTGTATATCCGAAAA TTAATGAGGGTGCTTTTTCTCATGTGATGGATTATAAGAGTCAGTTACAAGAATTGATTCAGCGTGATGG TAGTGGCAATGTTGAGTATCAAATTTTGCAAGAAAAAGGACCAGCTCACAATCGAGAATTTGTGTCACGT GTTACGTTAAATAACGTAGCTTTAGGTCTTGGTAGTGGTAAGTCGAAAAAAGAAGCAGAGCAACAAGCTG CTGCAGAAGCATTGAAAAAATTAAAAGAACAACTATAA Amino Acid B.cereus-E58A-aa B. cereus SEQ ID NO. 56 MPYRKYREKKYETKYREAFKVFQEKIGITFTDEKLLIQAFTHSSYVNEHRKKPHEDNARLEFLGDAVLEL TVSQYLFQKYPTMSEGELTKLRAAIVCEPSLVRFANELSFGSLVLLGKGEEMTGGRERPALLADVFEAFI GALYLDQGLETVWEFLKEIVYPKINEGAFSHVMDYKSQLQELIQRDGSGNVEYQILQEKGPAHNREFVSR VTLNNVALGLGSGKSKKEAEQQAAAEALKKLKEQL DNA B.subtilis-E59A B. cereus SEQ ID NO. 57 ATGTCAAAACACTCACATTATAAAGATAAAAAAAAGTTCTATAAAAAAGTAGAACAATTTAAAGAGTTTC AAGAACGGATTTCGGTTCACTTTCAAAATGAAAAGCTTTTGTATCAAGCATTTACACATTCATCTTATGT GAATGAGCATCGGAAAAAGCCGTATGAGGACAACGCTAGACTTGAATTTTTAGGTGACGCTGTTTTGGAA CTGACGATCTCCAGATTCTTATTTGCCAAATACCCGGCTATGAGTGAAGGAGATTTGACGAAATTGAGAG CCGCAATTGTTTGCGAACCGTCTCTCGTTTCATTGGCTCACGAGCTGTCATTCGGCGATCTTGTCCTGTT GGGTAAAGGCGAGGAAATGACAGGCGGAAGAAAGCGTCCTGCTCTATTGGCGGATGTTTTTGAGGCATTT ATCGGAGCCTTGTACCTTGACCAAGGATTAGAGCCGGTCGAAAGTTTCTTAAAAGTTTATGTGTTCCCTA AAATTAACGATGGTGCTTTTTCTCATGTGATGGATTTCAAAAGCCAGCTGCAGGAATACGTGCAGCGGGA CGGCAAAGGCTCTCTGGAGTATAAAATCTCCAACGAAAAAGGACCTGCGCACAACCGTGAATTTGAAGCC ATCGTATCTCTAAAAGGTGAACCACTCGGAGTCGGAAACGGCCGTTCAAAGAAAGAAGCCGAACAGCACG CTGCTCAGGAAGCTTTAGCTAAATTGCAAAAACACCATACGAAACAATAA Amino Acid B.subtilis-E59A-aa B. subtilis SEQ ID NO. 58 MSKHSHYKDKKKFYKKVEQFKEFQERISVHFQNEKLLYQAFTHSSYVNEHRKKPYEDNARLEFLGDAVLE LTISRFLFAKYPAMSEGDLTKLRAAIVCEPSLVSLAHELSFGDLVLLGKGEEMTGGRKRPALLADVFEAF IGALYLDQGLEPVESFLKVYVFPKINDGAFSHVMDFKSQLQEYVQRDGKGSLEYKISNEKGPAHNREFEA IVSLKGEPLGVGNGRSKKEAEQHAAQEALAKLQKHHTKQ DNA B.cereus-E137K B. cereus SEQ ID NO. 59 ATGCCGTACCGAAAATATAGAGAAAAAAAATACGAAACAAAATATCGTGAAGCATTTAAAGTGTTTCAAG AAAAGATAGGTATTACGTTTACAGATGAAAAATTATTGATTCAAGCATTTACGCATTCATCGTATGTGAA TGAGCATCGAAAAAAACCGCATGAAGATAATGAGCGTCTTGAATTTCTTGGAGATGCAGTATTGGAACTT ACTGTATCGCAGTATCTGTTTCAAAAATATCCGACAATGAGCGAAGGAGAGTTAACAAAACTACGTGCAG CTATTGTATGTGAGCCATCTCTTGTTCGTTTTGCGAACGAATTGTCATTTGGTAGCCTTGTTTTATTAGG AAAAGGTGAAGAAATGACAGGTGGACGTGAACGACCAGCTTTATTAGCGGATGTCTTCAAGGCCTTCATC GGTGCCCTTTATCTTGATCAAGGGTTAGAAACAGTTTGGGAATTCTTAAAAGAAATTGTATATCCGAAAA TTAATGAGGGTGCTTTTTCTCATGTGATGGATTATAAGAGTCAGTTACAAGAATTGATTCAGCGTGATGG TAGTGGCAATGTTGAGTATCAAATTTTGCAAGAAAAAGGACCAGCTCACAATCGAGAATTTGTGTCACGT GTTACGTTAAATAACGTAGCTTTAGGTCTTGGTAGTGGTAAGTCGAAAAAAGAAGCAGAGCAACAAGCTG CTGCAGAAGCATTGAAAAAATTAAAAGAACAACTATAA Amino Acid B.cereus-E137K-aa B. cereus SEQ ID NO. 60 MPYRKYREKKYETKYREAFKVFQEKIGITFTDEKLLIQAFTHSSYVNEHRKKPHEDNERLEFLGDAVLEL TVSQYLFQKYPTMSEGELTKLRAAIVCEPSLVRFANELSFGSLVLLGKGEEMTGGRERPALLADVFKAFI GALYLDQGLETVWEFLKEIVYPKINEGAFSHVMDYKSQLQELIQRDGSGNVEYQILQEKGPAHNREFVSR VTLNNVALGLGSGKSKKEAEQQAAAEALKKLKEQL DNA Ecoli-tetsac Artificial SEQ ID NO. 62 GAACTGTTGCAGCAGGCATTAACTCATCGTAGTGCCAGCAGTAAACATAACGAGTCCTAATTTTTGTTGA CACTCTATC DNA Ecoli-tet-sacB38R1 Artificial SEQ ID NO. 63 CGCATTGGCGATAACGTAGCTCAGAATAGAGTCGCCTAAAAATTCTAAACGATCAAAGGGAAAACTGTCC ATATGC DNA Ecoli-oligo-E38A Artificial SEQ ID NO. 64 GTAGCTCAGAATAGAGTCGCCTAAAAATTCGAAGCGGGCATTGTGTTTACTGCTGGCACTACGATGAGTT AATGC DNA Ecoli-E38A-1F Artificial SEQ ID NO. 65 AGTAAACACAATGCCCGCTTC DNA Ecoli-E38A-1R Artificial SEQ ID NO. 66 ATGCTTCGACGGTGTCGG DNA Ecoli-tet-sacB117F1 Artificial SEQ ID NO. 67 CTTAAAAGCGGTGGATTTCGTCGTGAGTCAATTCTCGCCGACACCGTCGAATCCTAATTTTTGTTGACAC TCTATC DNA Ecoli-tet-sacB117R1 Artificial SEQ ID NO. 68 TAATTTCTCGACGGTTTGAATATCACTGTCGAGGAATACGCCACCAATTAATGCATCAAAGGGAAAACTG TCCATATGC DNA Ecoli-oligo-E117K Artificial SEQ ID NO. 69 TTGAATATCACTGTCGAGGAATACGCCACCGATGAAAGCCTTCACGGTGTCGGCGAGAATTGACTCACGA CGAAA DNA Ecoli-E117K-1F Artificial SEQ ID NO. 70 GACACC GTGAAGGCTTTCATC DNA Ecoli-E117K-1R Artificial SEQ ID NO. 71 TTCAACGCCTGTTCGGC DNA Ecoli-oligo-E38A-F2 Artificial SEQ ID NO. 72 GTAGCTCAGAATAGAGTCGCCTAAAAATTCCAAGCGGGCATTGTGTTTACTGCTGGCACTACGATGAGTT AATGC DNA Ecoli-E38A-2F Artificial SEQ ID NO. 73 AGTAAACACAATGCCCGCTTG DNA Ecoli-oligo-E117K-F2 Artificial SEQ ID NO. 74 TTGAATATCACTGTCGAGGAATACGCCACCGATCAAAGCCTTCACGGTGTCGGCGAGAATTGACTCACGA CGAAA DNA Ecoli-E117K-2F Artificial SEQ ID NO. 75 GACACCGTGAAGGCTTTGATC DNA Ecoli-tet-sacB-E65F1 Artificial SEQ ID NO. 76 AGCTACGTTATCGCCAATGCGCTTTATCACCGTTTCCCTCGTGTGGATGAATCCTAATTTTTGTTGACAC TCTATC DNA Ecoli-tet-sacB-E65R1 Artificial SEQ ID NO. 77 CGCCAGCGTATTGCCACGGACCAGCGTGGCGCGCATCCGGCTCATATCGCCATCAAAGGGAAAACTGTCC ATATGC DNA Ecoli-oligo-E65A-F1 Artificial SEQ ID NO. 78 CAGCGTGGCGCGCATCCGGCTCATATCGCCGGCGTCGACGCGGGGGAAACGGTGATAAAGCGCATTGGCG ATAAC DNA Ecoli-E65A-1F Artificial SEQ ID NO. 79 TTTCCCCCGCGTCGACGC DNA JD-5 Artificial SEQ ID NO. 80 ACCGGTAAACTGAAACTGCA DNA Tet-sacB-JD-R1 Artificial SEQ ID NO. 81 TGGCAAGACTGGCATGATAAG DNA JD-3 Artificial SEQ ID NO. 82 TGGAGATTTTCTGCCCCAG RNA TMVU1-MP-F6-RNA21 Artificial SEQ ID NO. 83 CAGUUCAAGGUCGUUCCCAAU RNA TMVU1-MP-F7-RNA23 Artificial SEQ ID NO. 84 UGAAGAUGUCAGCGGGUUUCUGU RNA TMVU1-MP-R6-RNA25 Artificial SEQ ID NO. 85 CCAGACGUUUUUCAUCGCGUCCUGG RNA TMVU1-MP-R7-RNA27 Artificial SEQ ID NO. 86 ACGACUUCUUCUGUAAGUUCCAUGGGC RNA TMVU1-MP-F6-RNA29 Artificial SEQ ID NO. 87 CAGUUCAAGGUCGUUCCCAAUUAUGCUAU DNA Pveg-F1 Artificial SEQ ID NO. 88 ATCACGAGGCCCTTTCGTCTTCAAGGGAGTTCTGAGAATTGGTATGC DNA Pveg-R1 Artificial SEQ ID NO. 89 ACACCTCCTTTACTACATTTATTGTACAACACGAGC DNA Pveg-F2 Artificial SEQ ID NO. 90 ATCACGAGGCCCTTTCGTCTTCAAGAAGCTTGGAGTTCTGAGAATTGGTATGC DNA Pveg-R2 Artificial SEQ ID NO. 91 ACGCGATCCCCGGGTACCGAGCTCGCTCGAGACACCTCCTTTACTACATTTATTGTACAACACGAGC DNA Bc-E58A-F1 Artificial SEQ ID NO. 92 ACAATAAATGTAGTAAAGGAGGTGTATGCCGTACCGAAAATATAGAG DNA Bc-E58A-R1 Artificial SEQ ID NO. 93 GAGGCGGGCGTTGTCTTCATGCGGTTTTTTTCG DNA Bc-E58A-F2 Artificial SEQ ID NO. 94 ACCGCATGAAGACAACGCCCGCCTCGAATTTCTTGGAGATGCAGTATTG DNA Bc-E58A-R2 Artificial SEQ ID NO. 95 ACGCGATCCCCGGGTACCGAGCTCGTTATAGTTGTTCTTTTAATTTTTTCAATG DNA Bc-E137K-R1 Artificial SEQ ID NO. 96 GATGAAGGCCTTGAAGACATCCGCTAATAAAGCTGG DNA Bc-E137K-F1 Artificial SEQ ID NO. 97 AGCGGATGTCTTCAAGGCCTTCATCGGTGCCCTTTATCTTGATCAAG DNA pAD-E58A-F1 Artificial SEQ ID NO. 98 CAATAAATGTAGTAAAGGAGGTGTCATGCCGTACCGAAAATATAGAG DNA pAD-E58A-Artificial SEQ ID NO. 99 GCGAGCTCGGTACCCGGGGATCGCGTTATAGTTGTTCTTTTAATTTTTTCAATG DNA Eco-F1 Artificial SEQ ID NO. 100 ACGAGGCCCTTTCGTCTTCAA DNA SglyA-R1 Artificial SEQ ID NO. 101 CATGTTCGCTTGTGCACCA DNA Ae-JD-5 Artificial SEQ ID NO. 102 AACTAACGACATCCCCTGTCGT DNA Ae-JD-3 Artificial SEQ ID NO. 103 CGCAGCTTGTTCAGCACCAT DNA TMVMP-probe1s Artificial SEQ ID NO. 104 TCTCGGATCTTACTACACAGCAGCTGCAAAGAAAAGATTTCAGTT DNA TMVMP-probe2as Artificial SEQ ID NO. 105 TCCTGGGTGGTTATAGCATAATTGGGAACGACCTTGAACTGAAAT DNA TMVMP-probe3s Artificial SEQ ID NO. 106 CACCCAGGACGCGATGAAAAACGTCTGGCAAGTTTTAGTTAATAT DNA TMVMP-probe4as Artificial SEQ ID NO. 107 AGCGGACAGAAACCCGCTGACATCTTCACATTTCTAATATTAACT DNA TMVMP-probe5s Artificial SEQ ID NO. 108 CTGTCCGCTTTCTCTGGAGTTTGTGTCGGTGTGTATTGTTTATAG DNA TMVMP-probe6as Artificial SEQ ID NO. 109 CCCTCCGTCTCTCACGTTTGTAATCTTCTCTCTCAAACCTAATTT DNA TMVMP-probe8as Artificial SEQ ID NO. 110 CTTTGCAAGCCTGATCGACATAGGGACATCTTCCATGAACTCATC DNA TMVMP-probe9s Artificial SEQ ID NO. 111 GTTTCGATCTCGAACCGGAAAAAAGAGTGATGTCCGCAAAGGGAA DNA TMVU1-MP-F6-21 Artificial SEQ ID NO. 112 CAGTTCAAGGTCGTTCCCAAT DNA TMVU1-MP-R6-21 SEQ ID NO. 113 GTTTTTCATCGCGTCCTGGGT DNA TMVU1-MP-F7-21 Artificial SEQ ID NO. 114 AAGATGTCAGCGGGTTTCTGT DNA TMVU1-MP-R7-21 Artificial SEQ ID NO. 115 CTTCTTCTGTAAGTTCCATGG DNA TMVU1-MP-F7-21 Artificial SEQ ID NO. 116 AAGATGTCAGCGGGTTTCTGT DNA TMVU1-MP-R7-21 Artificial SEQ ID NO. 117 CTTCTTCTGTAAGTTCCATGG DNA TMVU1-MP-F4 Artificial SEQ ID NO. 118 CCAGGACGCGATGAAAAACG DNA TMVU1-MP-R4 Artificial SEQ ID NO. 119 GGACAGAAACCCGCTGACAT DNA Ec-16SrRNA-F1 Artificial SEQ ID NO. 120 GAATGCCACGGTGAATACGTT DNA Ec-16SrRNA-R1 Artificial SEQ ID NO. 121 ACCCACTCCCATGGTGTGA